Luc MONTAGNIER

DNA "Teleportatation"



Hypothesizes that that water formed a nano-structure & was able to emit an EM signal similar to the original DNA. The water nano-structures also were able to amplify into actual DNA strands.

See also : J. BENEVISTE / Digital Biology & Petr GAJAREV & V. POPONIN / DNA Reprogramming



http://www.pcworld.com/article/216767/dna_molecules_can_teleport_nobel_winner_says.html?tk=hp_new

Jan 16, 2011

DNA Molecules Can 'Teleport,' Nobel Winner Says

By John E Dunn, Techworld.com



http://arxiv.org/PS_cache/arxiv/pdf/1012/1012.5166v1.pdf

DNA Waves & Water



[ PDF ]



US8405379

System and method for the analysis of DNA sequences in biological fluids



WO2012142568

US2012024701

REMOTE TRANSMISSION OF ELECTROMAGNETIC SIGNALS INDUCING NANOSTRUCTURES AMPLIFIABLE INTO A SPECIFIC DNA SEQUENCE













Method of Detecting Microorganisms with a Specimen

US2010323391



Abstract

Description

EXAMPLE 1

A Lightly Dilute Bacterial Culture, not Emitting Electromagnetic Signals, "Negates" the Electromagnetic Signals Emitted by a Strong Dilution from the Same Culture

1) Sample Preparation

[0000] 2) Selection of Diluted Samples Generating Electromagnetic signals.

EXAMPLE 2

Quick and Non-Invasive Method for Detecting Infections in Humans and Animals

1) Preparations of Biological and Artificial Fluid Samples Containing Microorganisms.

2) Selection of Diluted Samples Generating Electromagnetic Signals.

3) Evaluating an Infected Individual's Inhibitory Activity on the Electromagnetic Signal Emission Generated by a Microorganism.

FIG. 2

FIG. 3





FIG. 4

FIG. 5

FIG. 6

FIG. 7

FIG. 8







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A Nobel Prize winning biologist has ignited controversy after publishing details of an experiment in which a fragment of DNA appeared to 'teleport' or imprint itself between test tubes.According to a team headed by Luc Montagnier, previously known for his work on HIV and AIDS, two test tubes, one of which contained a tiny piece of bacterial DNA, the other pure water, were surrounded by a weak electromagnetic field of 7Hz.Eighteen hours later, after DNA amplification using a polymerase chain reaction, as if by magic the DNA was detectable in the test tube containing pure water.Oddly, the original DNA sample had to be diluted many times over for the experiment to work, which might explain why the phenomenon has not been detected before, assuming that this is what has happened.The phenomenon might be very loosely described as 'teleportation' except that the bases project or imprint themselves across space rather than simply moving from one place to another.To be on the safe side, Montagnier then compared the results with controls in which the time limit was lowered, no electromagnetic field was present or was present but at lower frequencies, and in which both tubes contained pure water. On every one of these, he drew a blank.The quantum effect - the imprinting of the DNA on the water - is not in itself the most contentious element of the experiment, so much as the relatively long timescales over which it appears to manifest itself. Quantum phenomena are assumed to show their faces in imperceptible fractions of a second and not seconds minutes and hours, and usually at very low temperatures approaching absolute zero.Revealing a process through which biology might display the underlying 'quantumness' of nature at room temperature would be startling.Montagnier's experiment will have to be repeated by others to have any hope of being taken seriously. So far, some scientists have been publically incredulous."It is hard to understand how the information can be stored within water over a timescale longer than picoseconds," said the Ruhr University in Bochum's Klaus Gerwert, quoted by New Scientist magazine, which broke the story (requires registration).What does all of this mean? It could be that the propagation of life is able to make use of the quantum nature of reality to project itself in subtle ways, as has been hinted at in previous experiments. Alternatively, it could be that life itself is a complex projection of these quantum phenomena and utterly depends on them in ways not yet understood because they are incredibly hard to detect.Speculatively, (and Montagnier doesn't directly suggest anything so unsubstantiated), it could also be the little-understood quantum properties of the water molecule and not just its more obvious chemical bonding properties that gives it such a central role in the bio-engineering of life-forms. Water might be a good medium in which DNA can copy itself using processes that hint at quantum entanglement and 'teleportation' (our term).Montagnier's paper goes on to discuss the phenomenon he claims to have uncovered using 'quantum field theory' within the context of his personal interest, disease propagation.A general method for identifying both known and unknown DNA sequences at the origin of EMS, including DNA sequences in the plasma of patients suffering of chronic diseases such as Alzheimer, Parkinson, multiple sclerosis, rheumatoid arthritis, and other similar diseases, disorders and conditions. The invention is based on the discovery that: (1) The nanostructures induced by DNA sequences in water or other dipole solutions can faithfully reflect the information contained in these sequences at dilutions which do not contain anymore of that DNA, as evidenced by the fact that it can be retranscribed into the same DNA sequence by the polymerases and reagents used in classical polymerase chain reaction (PCR); (2) this information can be transmitted at a distance in water or other dipole solutions by EMS emitted by the nanostructures; and (3) EMS signatures of nanostructures containing this information can be detected, stored, transmitted, transduced and imprinted in water or other dipole solutions.[0005] Induction, detection and transmission of electromagnetic signals (EMS) from self-replicating molecules like DNA. Transduction of EMS from an EMS positive (EMS+) sample to a naïve, unsignalized sample. Methods for identifying a molecule like DNA in a sample by transducing its EMS signature to water, amplifying the signalized water to produce a DNA. Methods for detecting DNA associated with a condition, disorder or disease of incomplete or unknown etiology by inducing specific EMS emission from the sample at a particular frequency, signalizing a naïve sample with the emitted EMS, and detecting an EMS in the signalized water and/or amplifying the signalized water using a DNA amplification technique and analyzing the products of the amplification.[0007] The inventors have previously described a method for selectively detecting DNA sequences of pathogenic microorganisms by their emission of low frequency electromagnetic waves (EMS) in water dilutions. U.S. application Ser. No. 12/560,772, filed Sep. 16, 2009, entitled "System and Method for the Analysis of DNA sequences in Biological Fluids" discloses a method for detecting electromagnetic waves derived from bacterial DNA, comprising extracting and purifying nucleic acids from a sample; diluting the extracted purified nucleic acids in an aqueous solvent; measuring a low frequency electromagnetic emission over time from the diluted extracted purified nucleic acids in an aqueous solvent; performing a signal analysis of the low frequency electromagnetic emission over time; and producing an output, based on the signal analysis, in dependence on the DNA in the sample. The products and procedures as well as other subject matter disclosed in this patent application are expressly incorporated by reference.[0008] Methods for detecting some low electromagnetic frequency electromagnetic signals in diluted filtrates of the culture medium of certain bacteria and viruses, as well as in diluted plasma of patients infected by the same agents are disclosed by U.S. application Ser. No. 12/097,204, PCT/FR2007/001042, filed Jun. 22, 2007, and U.S. application Ser. No. 12/797,826, filed Jun. 10, 2010 each of which expressly incorporated by reference in their entirety. The electromagnetic signals (EMS) were believed to be produced by certain defined nanostructures induced by the microorganism, in high dilutions in water, after the microorganism had been removed by filtration.[0009] Materials and methods for detecting replicating molecules such as DNA and methods for EMS detection as well as other subject matter pertinent to the present invention disclosed in these documents is incorporated by reference to the following documents:[0023] In some instances, it was demonstrated that the EMS could originate from specific genes or even from some fragmented DNA sequences. This was discovered to be the case for the adhesin gene of Mycoplasma pirum (U.S. Ser. No. 12/097,204, filed Dec. 14, 2006) and of the LTR (Long terminal repeat), nef and pol genes of Human Immunodeficiency Virus (HIV) (U.S. 61/186,610, filed Jun. 12, 2009 & U.S. Ser. No. 12/797,826, filed Jun. 10, 2010). However, for many microbial agents or diseases of unknown origin or etiology this identification was not possible. Consequently, the inventor developed new methods, disclosed herein for detecting and identifying biological molecules, specifically DNA or other nucleic acids, associated with these other disease or disorders.[0024] There are several nonlimiting aspects to the invention.[0025] (1) A method for producing a solution, such an aqueous solution like water that contains nanostructures that characterize a molecule like DNA. This method involves dilution, usually serial dilution, of a sample containing DNA and agitation of the sample between dilutions to produce the water nanostructures.[0026] (2) Measuring EMS characteristic of a molecule like DNA or of its nanostructure in an originating sample and transducing this signal into a second receiving sample, usually water that does not emit the EMS signal. This is performed without contacting the originating sample and the receiving sample.[0027] (3) Electronic transmission of a detected or recorded EMS signal to a remove location and optionally imprinting it on a naïve sample and/or recovering DNA or other replicating molecule from the imprinted naïve sample.[0028] (4) Detecting DNA or DNA like molecules in a sample suspected of containing a particular agent, like HIV or Borellia.[0029] (5) Identifying DNA or similar molecules present in an unknown sample, such as from a sample from a subject having a disease of unknown etiology.[0030] (6) Devices that detect, induce, transduce or transmit EMS signals.[0037] Definitions:[0038] Nucleic acid: Includes single stranded, double stranded DNA, and RNA as well as modified polynucleotide sequences. Biological samples containing DNA associated with a disease or disorder are generally isolated or recovered in double stranded form.[0039] Self-replicating molecule: A molecule, such as DNA, that under appropriate conditions, can reproduce the information content of its primary, second, tertiary or quaternary structure. For example, a DNA molecule can replicate itself in the presence of the appropriate enzymes, primers and nucleotides.[0040] DNA Amplification: Methods for amplifying nucleic acids are known. Conventional methods including polymerase chain reaction (PCR) are known and are also incorporated by reference to Current Protocols in Molecular Biology (updated Apr. 5, 2010), Print ISSN: 1934-3639; Online ISSN: 1934-3647.[0041] Nanostructures: These structures of water are induced by biological molecules like nucleic acids such as single stranded or double stranded DNA. While not being bound to any particular theory, according to the physical theory of diphasic water, filtration and mechanical agitation (succussion) are believed to induce in water a low energy potential favoring the formation of quantum coherent domains. These domains will become replicas of a DNA molecule and vibrate by resonance when properly diluted and excited; see Del Guidice, et al., Water as a Free Electric Dipole Laser, Phys. Rev. Lett. 61, 1085-1088 (1988). Hydrogen bonding networks in liquid water, such as those described by Cowan, et al., Nature 434 (7030): 199-202 (2005) have not been associated with nanostructures.[0042] Serial Dilutions: Serial dilution is a well-known technique and involves the stepwise dilution of a substance, such as DNA, in a solvent, such as water, saline solution, aqueous buffer, or an aqueous alcohol solution. Generally, serial dilutions as performed herein are stepwise dilutions by a factor of 10, or dilution of 1 part of a more concentrated solution in 9 parts of a solvent.[0043] EMS: Electromagnetic signal. EMS in the context of the methods herein generally involves those having frequencies ranging from 0 Hz to 20,000 Hz as well as all intermediate subranges and values. Components of the ambient electromagnetic field include Schumann resonances which represent a set of spectrum peaks in the extremely low frequency (ELF) portion of the Earth's electromagnetic field spectrum. Schumann resonances are global electromagnetic resonances excited by lightning discharges in the cavity formed by the Earth's surface and the ionosphere and are the principal background in the electromagnetic spectrum between 3 and 69 Hz. A representative Schumann resonance peak occurs in the Earth's electromagnetic spectrum and an ELF of about 7.83 Hz. By comparison, 60 Hz cycling of electricity is used in North America and 50 Hz elsewhere in the world.[0044] EMS detection. Any suitable means for interrogating a sample and measuring its EMS may be employed. Exemplary systems, methods, and apparatuses for this purpose are disclosed by Butters, et al., WO 03/083439 A2, and are incorporated by reference to this document. Generally, these procedures will involve placing a sample into a container having electromagnetic and magnetic shielding, a source of Gaussian noise for injection in to the sample, a detector for detecting an electromagnetic time-domain signal composed of sample source radiation superimposed on the injected Gaussian noise, and a storage device for storing the time-domain signal and a time-domain signal separately detected from the same of a similar sample.[0045] EMS Signature: The EMS characteristic of a particular biological molecule or a time domain signal associated with a material of interest. EMS signatures for various biological molecules are disclosed by U.S. Ser. No. 12/797,826, filed Jun. 10, 2010. Such EMS signatures as well as methods for producing samples suitable for EMS detection and methods for detecting an EMS signature are incorporated by reference to this patent application.[0046] An EMS Signature of a particular molecule can be represented by a characteristic electromagnetic time domain signal. An EMS Signature may be recorded and replayed, undergo signal transformation or processing, or be transmitted.[0047] Excitation Frequency: A frequency used to excite a sample in which an EMS signature has been detected and induce an EMS signature in a sample previously devoid of the EMS signature, e.g., pure water. These frequencies include those of 7 Hz or above, e.g., 7, 8, 9, 10, 11, 12, 13, 14, 15, 20, 30, 40, 45, 50, 55, 60, 65, 70 or more.[0048] Originating Sample: A biological sample that contains an EMS signature, such as one characteristic of one or more biomolecules. An example would be a sample containing an EMS signature characteristic of DNA derived from human immunodeficiency virus.[0049] Receiving or Signalized Sample: A sample, such as water or another aqueous buffer or dipole that has acquired or been imprinted with a nanostructure corresponding to a biological molecule, such as DNA. Methods for producing signalized water by serial dilution and agitation in water or in an aqueous solvent are disclosed herein.[0050] Pathogenic Disease: Disease caused by or associated with a pathogen, such as a pathogenic parasite, yeast or fungus, bacterium, virus or infectious protein, such as a prion. Examples include parasitic diseases such as malaria or trypanosomiasis, fungal diseases, such as infections caused by or associated with Aspergillus, Candida, Histoplasma, Pneumocystis, Cryptococcus, Stachybotrys (black mold), bacterial infections such as Lyme Disease, sexually transmitted bacterial infections, tuberculosis, viral infections, including HIV infection, herpes virus infection, or hepatitis, and prion associated diseases such as Creutzfeldt-Jakob disease and so-called Mad Cow disease.[0051] Autoimmune Disease, Degenerative Disease, Disorders or Conditions: These diseases, disorders or conditions may or may not have been previously associated with a particular biological molecule, such as a particular DNA molecule or its corresponding water nanostructure. Examples include allergic conditions, multiple sclerosis, rheumatoid arthritis, disorders associated with transplantation or replacement of body parts, Alzheimer's disease, Parkinson's disease and other diseases or disorders of unknown or incomplete etiology, such as Chronic Fatigue Syndrome, Gulf War Syndrome, or with exposure to particular biological, chemical or physical agents or with the sequela of such exposure.[0052] Representative embodiments of the invention are described below.[0053] (i) Originating and Signalized Samples.[0054] Test samples used to produce an EMS will contain DNA or other replicating biological molecules that can form nanostructures or can be naïve samples signalized by EMS transduction to emit EMS or contain nanostructures representative of the DNA or other molecule. Representative test samples include blood, plasma, serum, CSF, joint fluid, saliva, mucous, semen, vaginal fluid, sweat, urine, and feces. Tissue samples and samples from other sources, including laboratory or hospital sources, foods, drinks and potable water may be used. These may be diagnostic samples, such as those obtained from a subject known to have or suspected of having a particular conditions, disorder or disease like AIDS or Lyme disease. Alternatively, they may be obtained from subjects having or suspected of having a condition, disorder or disease of unknown etiology, such as a parasitic or fungal disease or disorder, bacterial disease or disorder viral disease or disorder, an autoimmune disease, disorder or condition, diseases such as Alzheimer's Disease or Parkinson's Disease.[0055] To produce a sample that emits detectable EMS, a test sample undergoes dilution, usually serial dilution, and agitation preferably between each serial dilution. A test sample is usually diluted by a factor of 10<3>, 10<4>, 10<5>, 10<6>, 10<7>, 10<8>, 10<9 >10<10>, 10<11>, 10<12>, 10<13 >or more. Though any intervening factor of dilution or other degrees of dilution that produce detectable EMS may also be used. The beginning concentration of a nucleic acid in a sample prior to dilution generally ranges from 1 ng/ml to 4 ng/ml.[0056] Solutions for dilution and agitation as well as for containing an originating or receiving sample are preferably water, but other aqueous or dipolar solutions may be employed so long as they can provide nanostructures representative of DNA or other replicating molecules or induce detectable EMS when used. Examples of solutions include water, or other aqueous solutions, such as normal saline, phosphate buffered saline, physiologically acceptable aqueous solutions, buffered aqueous solutions, or alcohol and water mixtures, including 10, 20, 30, 40, 50, 60 and 70% or more of ethanol or other alcohol solutions or other solvents selected on a basis of their relevant properties depending on the molecule to be tested, may be employed in the methods described herein.[0057] In some applications, control samples are required. The type of control sample may be selected by one of skill in the art depending on the particular application but in general will not emit the EMS signature of the molecule of interest or contain nanostructures corresponding to it. Often, such controls will constitute pure, unsignalized water, distilled water or pyrolyzed water or other solutions known to be nucleic acid free.[0058] Signalized samples or solutions producing an EMS signature should not be boiled, heated or frozen for long periods of time so as to preserve the EMS signatures or nanostructures they contain. Preferably, these samples or solutions should be stored above freezing and less than 40[deg.] C.[0059] Various forms and time periods for agitation are contemplated and are incorporated by reference to the documents mentioned above. Vortexing for a period of 15 seconds between serial dilutions is one representative method for producing a sample emitting detectable EMS.[0060] (ii) EMS Transduction. The invention also relates to a method for producing an EMS signature in an aqueous buffer comprising placing an originating (EMS+) sample in an aqueous buffer and a receiving sample not having the EMS signature next to each other inside of an electromagnetically shielded container, applying an electromagnetic field for a time and under conditions sufficient to transfer the EMS signature from the originating sample to the receiving sample. The electromagnetic field is generally applied by a coil, such as a copper coil, located inside of an electromagnetically shielded container. Coils made of other electrically conducting metals or alloys may be employed or other devices that produce similar electromagnetic flux. The electromagnetic field can be applied to the sample for a time period ranging sufficient to produce an EMS signature, for example, from 12 to 24 hrs although other suitable time periods may be selected based on the nature of the sample, the sample dilution and the physical characteristics of the apparatus. Exposure time is chosen based on the amount of time required for transfer to occur. Some representative times include >0, 1, 2, 3, 4, 4-8, 8-12, 12-18, 18-24 and 24-48 hrs or longer. Signalized samples produced by this method as well as nucleic acids like DNA amplified from a signalized sample are also contemplated. Alternatively, an EMS signature may be imprinted in water or another aqueous buffer by contacting the one or more receiving samples with a recorded or transmitted and optionally amplified EMS signature previously obtained from an originating sample in an aqueous buffer having an EMS signature, for a time and under conditions sufficient to imprint the recorded or transmitted EMS signature of the originating sample onto the one or more receiving samples. Imprinting may be performed using means for applying an electromagnetic field, for example using a device, such as a copper coil or solenoid coil, optionally located inside of an electromagnetically shielded container. The electromagnetic field is applied to the sample for a time period sufficient to produce an EMS signature in the sample, for example for a period of 1 to 24 hrs. Other suitable time periods may be selected based on the nature of the sample, the sample dilution and the physical characteristics of the device or other means for applying the electromagnetic field. Signalized samples produced by this method as well as nucleic acids like DNA amplified from a signalized sample are also contemplated.[0061] (iii) EMS Recording/Transmission. EMS signals once measured may be recorded on a tangible medium, such as a computer hard drive, a flash drive, DVD, or CD or other known media. They may be transmitted electronically, for example, over the internet, or by any other means that preserves the signal integrity. Recorded or received signals can be amplified and used to transduce EMS into a naïve solution as described above. This aspect of the invention can involve the recording, transducing, storing, and/or transmission of an EMS signature of a nucleic acid, such as that produced after serial dilution of a signalized sample. An EMS signature may be recorded by a suitable electronic device, such as a recorder, computer or computer network. The recorded EMS signature may undergo signal processing or signal transformation for example into a digital or analog signal, be transmitted by a communications device, such as via radio, telephone, modem, or Internet transmission to a receiver, such as a receiving computer, anywhere in the world.[0062] A stored or transmitted EMS signature is then reconstituted and/or amplified and contacted with a receiving sample to imprint it with the EMS signature and produce nanostructures in the water or dipole solution of the receiving sample. Such a signal may be amplified prior to or after transmission, for example, using a commercial amplifier (e.g., Conrad). The electrical output from the amplifier containing the EMS signature is then applied to an electrically conducting coil (e.g., of copper wire) as described herein in which a plastic tube of pure non-signalized water or other dipole solution has been inserted for a time sufficient for imprinting of the EMS signature, generally for a period of at least one hour.[0063] The production of EMS is then verified in water dilutions of the signalized water or dipole solution. The positive dilutions can be used for retrieving the DNA by PCR as described above. The DNA is then amplified by cloning and its sequence determined to be 98-100% identical to the initial DNA. This development will be useful for remote diagnosis or use in other telemedicine procedures or protocols.[0064] The inventors previously discovered that an electromagnetic signal of low frequency (EMS) induced in a water dilution by the DNA of some kinds of bacteria and viruses can be transmitted at a distance into a naive or unsignalized water, aqueous medium or other dipole solution. It has also been discovered that such an EMS corresponding to a particular biomolecule like DNA (i.e., an EMS signature of a particular molecule), can be recorded. This involves recording EMS from DNA fragments obtained by PCR (polymerase chain reaction) with sequence specific primers in an electromagnetic coil. The resulting amplified current is connected to a computer and stored as a file, such as an analog or digital file (e.g., a digital sound file). The recorded EMS can then undergo signal processing, for example a digital sound file can be processed using computer software for storage, transmission, or use.[0065] DNA may be reconstituted from its EMS signature. For example, the recorded or remotely transmitted EMS signature of a DNA molecule is input into a soundcard and the output from the soundcard is linked to an amplifier. Amplifier output is connected to a transducer solenoid into which an unsignalized water sample is placed. After a certain time, depending on the type of EMS signature, its intensity and the exposure time, the unsignalized water becomes signalized. In other words, the unsignalized water has memorized the EMS signature of the originating DNA molecule. By use of PCR the originating DNA molecule may be retrieved from the water signalized with its EMS signature. Verification of retrieval of the originating DNA sequence from the signalized water or verification of the fidelity of its reproduction can be verified by DNA sequencing.[0066] Alternatively, prior to retrieval and synthesis of the DNA molecule by PCR, the signalization of the receiving sample with a DNA EMS signature may be determined by detecting the EMS emissions of the signalized sample using dilutions of the signalized water as previously described, e.g., by the device used to record the originating DNA sample's EMS signature in the first place. Only EMS positive dilutions will yield the DNA sequence. The procedure allows the transmission of DNA EMS signatures of medical interest as well as the remote retrieval of the corresponding originating DNA. Such transmission may be made by a medium of choice, for example, a digital signal may be transmitted over the internet or by sending USB keys (e.g., flashdrives) to remote laboratories or medical units.[0067] (iv) Detection of a Known Nucleic Acid Sequence. Specific molecules known or suspected to be contained in a test sample may be screened using the methods described above. A test sample is diluted and agitated to produce an EMS+ sample and a nucleic acid amplification using specific known primers for the nucleic acid sequence of interest is performed. The test sample may be a sample produced by dilution and agitation or may be produced by tranduction of EMS into a naïve sample. An EMS+ test sample is incubated with primers for a specific nucleic acid sequence and the nucleic acid product by PCR amplification, usually DNA, is recovered. The recovered amplification products may be assayed indicate the presence of the particular nucleic acid in the test sample.[0068] (v) Identification of an Unknown Nucleic Acid.[0069] Another embodiment of the invention involves detecting a nucleic acid or nanostructures associated with an unknown nucleic acid in a test sample comprising amplifying a nucleic acid in a test sample using random nucleotide sequence or polynucleotides or primers; diluting and agitating during dilution the amplified nucleic acids in an aqueous solvent; measuring over time a low frequency electromagnetic emission from the diluted amplified nucleic acids; and optionally (i) identifying an EMS signature for amplified nucleic acid or its associated nanostructures by comparing the EMS of the test sample to the EMS of a control sample, and optionally (ii) comparing the results to relevant standard EMS signature(s). This method may further comprise performing a signal analysis of the low frequency electromagnetic emission over time, and/or producing an output, based on the signal analysis. This method may detect a biological molecule, such as a nucleic acid like DNA in a test sample and/or may detect a nanostructure derived from or associated with a nucleic acid such as DNA in the test sample. A suitable dilution of the test sample is selected for use within this method, for example, the test sample can be diluted by a factor of at least 10<4>, 10<5>, 10<6>, 10<7>, 10<8>, or 10<9>.[0070] The test sample will usually be obtained from subject suffering from or at risk of developing a particular disease, disorder or condition. For example, the test sample can be obtained from a subject having or suspected of having a parasitic or fungal disease or disorder, a subject having or suspected of having a bacterial disease or disorder, a subject having or suspected of having viral disease or disorder, from a subject having or suspected of having had an autoimmune disorder, a subject having or suspected of having Alzheimer's Disease or Parkinson's Disease or any other neurological disease, a subject having or suspected to have a genetic disease or a gene alteration, or a subject having a disease, disorder or condition of unknown or incomplete etiology in comparison with a noninfected subject. For instance, an EMS signature of an HIV gene sequence, such as that of nef or pol, may be detected in a sample in comparison to a sample not containing the HIV gene sequence. Verification of the presence of a gene sequence in a sample may be made by PCR.[0071] (vi) Devices. Various devices for use in conjunction with the different aspects of the invention are also disclosed. These include:[0072] A device for producing an EMS signature in an aqueous buffer comprising at least two containers, at least one for an EMS originating sample and at least one for an EMS receiving sample, an electrically conducting coil that can emit a variable frequency ranging from 1 to 20,000 Hz, optionally connected to an external generator of alternating current having a variable frequency from 1 to 20,000 Hz, means for electromagnetic shielding the at least two containers and the electrically conducting coil.[0073] A device or other means for transmitting at a distance EMS emitted by a biological sample or by nanostructures contained in a sample is also contemplated. Such a device will contain at least two containers, at least one to contain a sample determined to produce EMS characteristic of a DNA or a similar molecule in a first tube (originating sample), and another tube (receiving sample) to receive emitted EMS and contain signalized water produced. The device will contain an electrically conducting coil linked to an external generator of alternating current having a variable frequency from 1 to 20,000 Hz. The device will have shielding means, such as mu metal >=1 mm in thickness, capable of isolating external ambient electromagnetic signals or noise, enclosing a space into which will accommodate the coil and the containers. Any suitable material may be used to make the coil and the elements and design of the coil are selected based on the size of the samples, shielding, and other elements of the apparatus. One example of a coil is a copper coil with the following characteristics: bobbin with internal diameter 50 mm, length 80 mm, R=3.6 ohms, 3 layers of 112 turns of copper wire, field on the axis to the centre 44 Oe/A, and on the edge 25 Oe/A. An example of shielding is a cylinder of [mu] metal having a minimal thickness of 1 mm, closed at both ends in a manner that completely isolates the enclosed containers and coil from the external ambient electromagnetic noise.[0074] The following Examples describe particular embodiments of the invention, but the invention is not limited to what is described in these Examples.[0075] Step A:[0076] Synthesis of DNA by PCR[0077] A particular DNA sequence is first synthesized by polymerase chain reaction (PCR) on a DNA template, for example, a region of the LTR sequence present in the viral DNA extracted from the plasma of a HIV infected patient or obtained from a purified infectious DNA clone of HIV1 Lai, is amplified by PCR and nested PCR with respectively LTR-derived outer and inner primers.[0078] Those were chosen to pick up some conserved regions of the LTR, given to several subtypes of HIV1. This amplified DNA was sequenced and found 100% identical to the known sequence of the prototype strain of HIV1 subtype B, HIV1 LAI (3). The resulting amplicon was determined to be 488 bp long and the nested-PCR amplicon to be 104 bp long.[0079] Filtration and Dilution: A sample of each amplicon is prepared at a concentration of 2 ng/ml in a final volume of 1 ml of pure water that had been previously filtered through a sterile 450 nM Millipore (Millex) filter and then to a 20 nM filter (Whatman, Anotop) to eliminate any contamination by viruses or bacteria. All manipulations are done under sterile atmosphere in a biological safety cabinet.[0080] The DNA solution is diluted one in 100 (10) in 2 ml of water and filtered through a 450 nM Millex filter (Millipore) and filtered again through an Anotop filter of porosity size 20 nM (Whatman).[0081] The resulting DNA filtrate (there is practically no DNA loss through filtration, as the DNA molecules do not bind to the filters), is then diluted serially 1 in 10 (0.1 ml in 0.9 ml of water in an Eppendorf sterile tube of 2 ml from 10to 10.[0082] A strong vortex agitation was performed at each dilution step for 15 seconds.[0083] Each dilution in its stoppered plastic tube was placed on a coil under the ambient electromagnetic background at room temperature for 6 seconds; the resulting electric current is amplified 500 times and analyzed in a Sony laptop computer with specific software as previously described. The EMS positive vibrating dilutions (usually between 10to 10) were detected not only by new peaks of frequency, but also quantitatively by the difference in amplitude and intensity of the signals measured in the software, as compared to the same parameters given by the background noise.[0084] Table 1 shows the role of excitation frequency in inducing EMS from DNA into water. A fragment of LTR DNA (Tar region, 104 base pairs) was amplified by PCR with specific primers from the entire genomic HIV1 LAI DNA cloned in a plasmid (pLAI2). The fragment was purified by electrophoresis on an agarose gel; the DNA band was then cut and extracted with a Qiagen kit. Time of exposure DNA tube and water tube to the exciting frequency was 18 hrs.[0000]TABLE 1PositiveContent Frequency (Hz) EMS % over noise dilutionsLTR DNA 104 bp 2 + 33.3 D6-> D8Water - 1.2DNA 3 + 39.6 D4-> D7Water - 0.5DNA 4 + 43.9 D5-> D8Water - 1.5DNA 5 + 41.6 D5-> D8Water - 0DNA 6 + 33.5 D5-> D8Water - 1DNA 7 + 40 D6-> D8Water + 43.9 D5-> D8[0085] Step B:[0086] Producing a Signalized Sample from the Originating Sample[0087] Tube 1 containing one of the dilutions found positive for EMS in step A (10) was placed in the vicinity of an identical tube 2 that had been previously filled with 1 ml of pure water under a separate safety cabinet different from the one utilized in step A for the DNA manipulation. Both tubes were placed inside a copper coil with the following characteristics: bobin with internal diameter 50 mm, length 80 mm, R=3.6 ohms, 3 layers of 112 turns of copper wire, field on the axis to the centre 44 Oe/A, and on the edge 25 Oe/A, linked to an external generator of alternate electric current of variable frequency from 1 to 20,000 Hz.[0088] The tubes and the coil were enclosed in a cylinder of thick (1 mm) [mu]metal closed at both ends in order to isolate the system from the external ambient electromagnetic noise. A current intensity of 100 mA was applied to the coil, so that no significant heat was generated inside the cylinder.[0089] The tubes were kept 18 Hrs at room temperature in an oscillating magnetic field strength of 25 Oe/A generated by the coil system. Afterwards, the signalized water of tube 2 is filtered on 450 nM and 20 nM filters and diluted from 10to 10. As a control, the tube 1 was also filtered and diluted in the same way. EMS analysis revealed positive dilutions for EMS, starting at 10which is explained if one takes into account that the emitter tube 1 was already at the 10dilution (FIG. 1). As shown in Table 1 a minimal frequency of 7 Hz was found necessary and sufficient to induce the EMS in the naïve, unsignalized water filled tube 2. However, the intensity of the EMS signals was sometimes reduced by comparison to those found in tube 1. To determine conditions suitable for EMS transduction, the inventors also varied different parameters of the process. It was determined that the following conditions suppressed EMS emission from naïve tube 2 (receiving sample or sample to be signalized).[0090] Time of exposure of the two tubes less than 16-18 hrs (Table 2).[0091] No coil.[0092] Generator of magnetic field turned off.[0093] Frequency of excitation<6 Hz.[0094] No use of DNA in tube 1.[0095] Tube 2 frozen at -80[deg.] C. overnight and defrosted before recording the EMS.[0096] Tube 2 heated at 95[deg.] C. for 60 minutes after the overnight exposure.[0097] Based on the results in Table 1 and on testing of the process conditions and parameters it was concluded that excitation of tube 1 by a magnetic field of low frequency and of very low intensity has allowed the water nanostructures generated by the DNA fragment contained in this tube to be transmitted via waves to tube 2.[0098] Step C:[0099] Reconstitution by PCR of the LTR DNA from the Nanostructures in the Receiving or Signalized Sample.[0100] A sample volume (5 [mu]l) of tube 2-signalized water was added to 45 [mu]l of an amplification mixture in a propylene 200 [mu]l PCR tube (Eppendorf).[0101] The amplification mixture was composed of (buffer composition) 0.2 mM dNTP's, 10 [mu]M of each specific HIV-1 LTR primer containing the ingredients for synthesizing DNA, either from a positive dilution for EMS or in a lesser dilution, starting with 10down to 10: and using 1 unit of Taq DNA polymerase.[0102] Once the first cDNA strand is synthesized, cycling of denaturation, annealing and polymerization steps are performed as usually used for the PCR amplification.[0103] The reaction (35 cycles, T[deg.] annealing 56[deg.] C.) yielded a DNA band of the size (in electrophoresis migration in agarose 1.5%) of the expected 104 bp sequence. This amplicon was then cloned in a bacterial plasmid (Topo Cloning, Invitrogen) which was used to transform bacterial competent cells. Plasmid clones were purified from isolated bacterial transformants and screened for the presence of the 104 bp insert by EcoRI digestion. Positive plasmid clones are then sequenced and the sequence of the insert shown to be 98% to 100% identical (difference of 2 nucleotides) to the original DNA of tube 1.[0104] The first step of DNA synthesis using the nanostructures as templates can also be achieved by a reverse transcriptase (RT) and other more classical DNA polymerase, at lower temperature (42[deg.] C. for example for the reverse transcription step). HIV1 LTR DNA D6 (EMS positive) dilution was used as emitter using excitation frequency of 7 Hz during 18 hours in the apparatus described in FIG. 1, and placed close to the water receiver Tube 2. Like the latter, it was then diluted at 10, refiltered by 450 nM and 20 nM filters and diluted to 10.[0105] Each dilution was then amplified by PCR for 35 cycles. Note the DNA bands detected at dilutions D2, (FD2), D3, D4, and D5. It has to be noted that the synthesis of the DNA LTR band is obtained in high water dilutions (up to 10) of the tube 2 containing the signalized water, indicating the transmission of the DNA information from tube to tube, in the presence of the ambient electromagnetic background. The same phenomenon was also observed in high dilutions of tube 1, indicating the synthesis of DNA at dilutions containing no DNA molecules.[0106] This PCR technology can be applied to the detection of nanostructures in body fluid (plasma, urine) apparently devoid of the microorganisms from which they originate. In all cases, it is necessary to use mechanical agitation (vortex) at each water dilution in addition to the ambient or controlled electromagnetic background.[0107] Table 2 shows the role of time of exposure to the 7 Hz frequency on EMS transmission from DNA to water. These results used the DNA LTR preparation as used for procedures reported in Table 1.[0000]Time of PositiveContent exposure (hr) EMS % over noise dilutionsControl DNA tube 2 + 57.3 D4-> D8Water 2 - 0Water 4 - 0Water 6 - 0Water 8 +- 6.4 D4-> D8Water 16 + 13.4 D5-> D8Control DNA tube 16 + 63 D4-> D8[0108] As shown above EMS were detected in the receiving sample after an exposure time of 8 or 16 hrs when the originating sample exhibited positive EMS at dilutions of D4 to D8 (10to 10). No EMS was detected in water exposed for less than 8 hrs.Identification of Unknown DNA Using Random Primers[0109] Another aspect of the invention is directed to a general procedure for the identification of any unknown DNA sequence (or polynucleotide sequence) capable of producing EMS in biological fluids. The principle is shown by FIG. 3. The transmission of EMS in water allows the selective transmission of only the DNA sequences that were emitting the EMS under the induction conditions. The PCR method uses a combination of random and Tag primers. The random primer associated with the Tag has the following formula 5'-GGACTGACGAATTCCAGTGACTNNNNNNNN (SEQ ID NO: 1) in which are made all possible combinations of 8 nucleotides for the 4 possible bases (65,536). A detailed procedure is described below.[0110] 1) DNA is purified from EDTA-collected human plasma extracted by the kit, QiaAMP, (Qiagen).[0111] 2) The purified DNA samples are filtered through 0.45 and 0.1 [mu]m filters and then diluted to FD2-FD15 for analysis of EMS. FD2 refers to a filtered dilution of 1:100 or 10.[0112] 3) The filtered and diluted samples are used to signalize water (molecular biology grade, 5Prime, 20 nm-filtered) with a dilution EMS+ of a patient DNA sample under an oscillating magnetic field of 7 Hz, 4V (coil in mu-metal) for 18 hours.[0113] 4) Each EMS+ sample used is filtered, vortexed and diluted (FD2-FD5) the signalized water sample and proceed to EMS analysis.[0114] 5) The samples of signalized water (EMS+), starting with FD2 are used as template for PCR amplification using random and Tag primers, following the protocol described below:[0115] A 49 [mu]l PCR amplification mix containing 1* Advanced Taq buffer with Mg<2+> (available from 5Prime Co.), 200 [mu]M dNTPs, 20 nM of designed random primer Tag8N (SEQ ID NO: 1):[0000](SEQ ID NO: 2)(5'-GGACTGACGAATTCCAGTGACTNNNNNNNN)[0116] 20 [mu]l of vortexed FD2 signalized water template, and 1 unit of Taq DNA polymerase (available from 5Prime Co.) is incubated stepwise at 8[deg.] C., 15[deg.] C., 20[deg.] C., 25[deg.] C., 30[deg.] C., 36[deg.] C., 42[deg.] C., and 46[deg.] C. for 2 min at each temperature to allow annealing of the random portion of the primer. An elongation step at 68[deg.] C. for 2-15 min was performed to allow synthesis of DNA, followed by a denaturation step at 95[deg.] C. for 3 min. One [mu]l of the designed primer Tag-ONLY (5'-GGACTGACGAATTCCAGTGACT) (SEQ ID NO: 3) is added to the mixture at a final concentration of 200 nM. The resulting sample is subjected to 40 cycles of amplification (95[deg.] C./30 s, 59[deg.] C./30 s, and 70[deg.] C./2 min), followed by an incubation at 70[deg.] C. for 10 min. PCR-amplified samples are subjected to electrophoresis in 1.3% agarose gel and stained with ethidium bromide to allow visualization of amplified DNA bands under UV light.[0117] 6) If needed (if faint or no DNA bands a-re detected), sample can be reamplified by PCR using only the primer Tag-ONLY, following the reamplification protocol described below:[0118] A 50 [mu]l PCR amplification mix containing 1* Hot Start Taq buffer with Mg<2+> (available from 5Prime Co.), 200 [mu]M dNTPs, 200 nM of designed primer Tag-ONLY (5'-GGACTGACGAATTCCAGTGACT) (SEQ ID NO: 3), 1-10 [mu]l of PCR-amplified sample as template, and 1 unit of Hot Taq DNA polymerase (available from 5Prime Co.) is denatured at 95[deg.] C. for 3 min and subjected to 25-40 cycles of amplification (95[deg.] C./30 s, 59[deg.] C./30 s, and 70[deg.] C./2 min), followed by an incubation at 70[deg.] C. for 10 min.[0119] 7) Isolation, purification and cloning of amplicons in pCR2.1-TOPO (InVitrogen) vector, followed by transformation of competent Escherichia coli cells, and screening for positive clones.[0120] 8) DNA sequencing of amplicons using M13 universal primers (Eurofins MWG GmbH, Germany) and BLAST of the resulting sequences.[0121] Application to a patient suffering from chronic Lyme disease:[0122] A D9 (10) dilution of DNA extracted from the plasma of a patient suffering from chronic Lyme disease was transduced into water at an excitation frequency of 7 Hz for 18 hrs. PCR was performed on the water sample after transduction with Tag8N primers followed by a second PCR with Tag primers only. The PCR DNA products were resolved on agarose gels by electrophoresis and are shown in FIG. 4. As shown at the left, results obtained when the tube of D9 DNA and the naive tube of water are placed side-by-side. At right, results obtained when the two tubes were placed at a distance of 4 cm from each other.[0123] Dw denotes control, naïve, unsignalized water.[0124] Dw vor: denotes control naïve, unsignalized water agitated with a vortex.[0125] D0: water that was transduced but not diluted.[0126] D2 NF: same as D0 but diluted by 1:100 (D2).[0127] D2 same as D2 NF, but filtered.[0128] D3, D4, D5 represent further serial dilutions of D2 to factors of 1:1,000 (D3); 1:10,000 (D4) and 1:100,000 (D5). All serial dilutions were vortexed between each 1:10 dilution.Recording and Transduction of EMS Signatures of HIV and Borrelia Burgdorferi[0129] EMS signatures of HIV DNA and Borrelia DNA sequences are recorded and transduced as described below.[0130] Step 1: Preparation of DNAs[0131] 1. A fragment of HIV DNA taken from its long terminal repeat (LTR) sequence present in the viral DNA extracted from the plasma of a HIV-infected patient or obtained from a purified infectious DNA clone of HIV1 Lai, is amplified by PCR (487 base pairs) and nested PCR (104 base pairs) using specific primers: TR InS 5'-GCCTGTACTGGGTCTCT (SEQ ID NO: 4) and LTR InAS 5'-AAGCACTCAAGGCAAGCTTTA (SEQ ID NO: 5). A longer variant (300 bp) is obtained using the following primer: 5'-TGTTAGAGTGGAGGTTTGACA (SEQ ID NO: 6) in conjunction with the above primer InAS.[0132] 2. A DNA sequence from Borrelia Burgdorferi, the agent of Lyme disease, is amplified by PCR (907 base pairs) and nested PCR (499 base pairs) with respectively Borrelia 16S outer and inner primers. Inner BORR16S inS 5'-CAATCYGGACTGAGACCTGC (SEQ ID NO: 7) and BORR16S inAS 5'-ACGCTGTAAACGATGCACAC (SEQ ID NO: 8). A shorter variant of 395 bp is obtained by using the following primer: 5'-GACGTCATCCTCACCTTCCT (SEQ ID NO: 9) in conjunction with the above primer inAS.[0133] Step 2: Signal Recording[0134] The resulting amplicons 104 bp and 300 bp for LTR and 499 bp and 395 bp for Borrelia were prepared at a concentration of 2 ng/ml in a final volume of 1 ml of DNAse/RNAse-free distilled water. The samples were read on an electromagnetic coil, connected to a Sound Blaster card (Creative Labs) itself connected to a microcomputer, (preferably Sony VGN-CS31) preferentially powered by its 12 volt battery. Each emission is recorded for 6 seconds, amplified 500 times and the digital file is saved, for example under the form of a sound file with the .wav format. This file can later undergo digital processing, by a specific software, Matlab (Mathworks), as for example digital amplification for calibrating the signal level, filtering for eliminating unwanted frequencies, or be analyzed by transformation into its spectrum by a discrete Fourier transform, preferably by the algorithm of FFT "Fast Fourier Transform".[0135] Step 3: Signal Transduction in Water:[0136] For transduction, the digital signal was converted by the digital/analog converter of the sound card into an analog signal. The output of the sound card of the microcomputer was linked to the input of a commercial amplifier (Kool Sound SX-250, www._conrad.com) having the following characteristics: passband from 10 Hz to 20 kHz, gain 1 to 20, input sensitivity 250 mV, output power RMS 140 W under 8 ohms.[0137] The output of the amplifier was connected to a transducer solenoid which has the following characteristics: the bobbin has a length of 120 mm, an internal diameter of 25 mm, an external diameter of 28 mm, with 3 layers of 631 spirals of copper wire of 0.5 mm diameter and a resistance of 8 ohms, field on the axis to the centre 44 Oe/A, and on the edge 25 Oe/A. A measurement of 4.4 milliTesla (mT) was obtained when current, voltage and resistance were respectively, 100 mA, 4V and 8 ohms.[0138] 50 ml of DNAse/RNAse-free distilled water (5-Prime Ref 2500010) are filtered first through a sterile 450 nM filter (Millex, Millipore, Cat N[deg.] SLHV033RS) and then to a 20 nM filter (Whatman, Anotop 25, Cat N[deg.] 6809-2002). For transduction, 1 ml of this filtered water in a Eppendorf sterile tube of 1.5 ml was placed at the center of the solenoid, itself installed at room temperature on an isolated (non metal) working bench. Alternatively, a sterile tube of 15 ml (Falcon-Becton Dickinson), filled with the filtered water can be used instead of the 1.5 ml Eppendorf tube.[0139] The modulated electric current produced by the amplifier was applied to the transducer coil for 1 hr at the tension of 4 Volts. A current intensity of 100 mA was applied to the coil, so that no significant heat was generated inside the cylinder.[0140] Step 4: Reconstitution by PCR of the DNA from the Signalized Water.[0141] The water which has received the recorded specific signal is called "signalized water". The signalized water (kept in the same tube) was first agitated by strong vortex for 15 seconds at room temperature and then diluted 1/100 in non signalized DNAse/RNAse-free distilled water (30 [mu]l/3 ml). 1 ml was kept for control (NF, nonfiltered), the 2 mls remaining of signalized water were filtered through a sterile 450 nM filter and then through a 100 nM (Millex, Millipore, Cat N[deg.] SLVV033RS) for Borrelia DNA or 20 nM filter (Whatman, notop25) for HIV DNA. The filtrate was then diluted serially 1 in 10 (0.1 ml in 0.9 ml of DNAse/RNAse-free distilled water) in a Eppendorf sterile tube of 1.5 ml from 10to 10(D2 to D15). A strong vortex agitation was performed at each dilution step for 15 seconds. 5 [mu]l of each dilution is added to 45 [mu]l of the mix.[0142] 1. Preparation of the mix for HIV LTR: The PCR mixture (50 [mu]l) contained 37.4 [mu]l of DNAse/RNAse-Free distilled water, 5 [mu]l of 10* Taq PCR buffer, 0.4 [mu]l of 25 mM dNTPs, 1 [mu]l of 50 [mu]M each appropriate primer Inner [LTR InS (5'-GCCTGTACTGGGTCTCT) (SEQ ID NO: 10) and LTR InAS (5'-AAGCACTCAAGGCAAGCTTTA) (SEQ ID NO: 11)], 0.2 [mu]l of 5 U/[mu]l Taq DNA Polymerase and 5 [mu]l of each dilution. The PCR was performed with the mastercycler ep (Eppendorf). The PCR mixtures were pre-heated at 68[deg.] C. for 3 min (elongation step), followed by 40 PCR cycles of amplification (95[deg.] C. for 30 s; 56[deg.] C. for 30 s; 70[deg.] C. for 30 sec). A final extension step was performed at 70[deg.] C. for 10 min.[0143] 2. Preparation of the mix for Borrelia: The PCR mixture (50 [mu]l) contained 37.4 [mu]l of DNAse/RNAse-Free distilled water, 5 [mu]l of 10* Taq PCR buffer, 0.4 [mu]l of 25 mM dNTPs, 1 [mu]l of 50 [mu]M each appropriate primer Inner [BORR16S inS (5'-CAATCYGGACTGAGACCTGC) (SEQ ID NO: 7) and BORR16S inAS (5'-ACGCTGTAAACGATGCACAC) (SEQ ID NO: 8)], 0.2 [mu]l of 5 U/[mu]l Taq DNA polymerase and 5 [mu]l of each dilution. The PCR was performed with the mastercycler ep (Eppendorf). The PCR mixtures were pre-heated at 68[deg.] C. for 3 min (elongation step), followed by 40 PCR cycles of amplification (95[deg.] C. for 30 s; 61[deg.] C. for 30 s; 70[deg.] C. for 1 min). A final extension step was performed at 70[deg.] C. for 10 min.[0144] Electrophoresis of the PCR products in 1.5% agarose gel: A band of 104 bp for HIV LTR and a band of 499 bp Borrelia DNA should be detected at several dilutions.[0145] 3. Sequencing: The DNA bands are cut and DNA is extracted using a Qiagen kit which also describes classical conditions for cloning in E. coli. The amplified specific DNA is then sequenced to show its identity to the original DNA.2010-12-23Inventor(s): MONTAGNIER LUC [FR]; AISSA JAMALClassification: - international: C12M1/34; C12Q1/04 - European: C12Q1/04; G01N37/00Also published as: FR2902883 // RU2009101670 // WO2007147982 // WO2007147982 // EP2044210-- This invention concerns a process for preparing reagents intended for a microorganism detection test and notably an infection in humans or animals, wherein the following steps are included: a) Centrifuging a biological or artificial liquid medium containing a selected specific microorganism; b) Filtrating the supernatant obtained in step (a); c) Preparing a series of diluted samples corresponding to increasing dilutions of the filtrate obtained in step (b), down to a filtrate dilution of at least a factor of 10-15; d) Submitting said diluted samples obtained in step (c) to an electrical, magnetic, and/or electromagnetic exciting field; e) Analyzing the electrical signals detected using a solenoid, as well as digitally recording said electrical signal after analog/digital conversion of said signal; f) Selecting diluted samples with which the characteristic electrical signals were obtained in (e), i.e. signals whose amplitude is at least 1.5 times greater than background noise emitted by water and/or presenting a frequency displacement towards higher values; g) Placing the diluted samples selected in step (f) into protective enclosures, which are protecting said dilutions against external electromagnetic fields; h) Distributing one of the aforesaid diluted samples from step (g), volume by volume, into two tubes, T1 and T2, tube T1 remaining in a protective enclosure protecting diluted samples from external electromagnetic field interferences, and acting as a reference solution, tube T2 being also placed in a protective enclosure, and subjected subsequently to the presence or contact of a sample suspected to contain said selected specific microorganism.[0001] This invention has for object to reveal latent infections in humans and animals, by showing inhibition, through the examinee, of electromagnetic signals generated by a microorganism.[0002] From the works by Dr. Jacques BENVENISTE and from patent application WO 00/17637, it has been known how to record and digitalize, after analog-to-digital conversion using a computer sound board, an electrical signal characteristic of a molecule possessing a biological activity.[0003] Also known in prior art (WO 09417406) is a process and a device used to transmit biological activity from a first matter, so-called carrier, to a second matter, so-called target, the latter exempted of any traces from said carrier and physically separate from it, and the target not presenting initially the aforementioned biological activity. The method consists in (i) exposing the matter carrying the biological activity of interest to an electrical or electromagnetic signal sensor, (ii) amplifying said electromagnetic or electrical signals characteristic of the emitted biological activity feature, then (iii) exposing the target matter to an emitter of electrical or electromagnetic signals, said emitter being connected to aforesaid sensor through a transmission and amplification circuit, in order to transmit the signal characteristic of biological activity to said target.[0004] In a previous French patent application 05/12686 filed on Dec. 14, 2005, not yet issued to this day, the inventor of this invention was describing a process for characterizing biochemical elements presenting a biological activity, microorganisms in this case, by analyzing low frequency electromagnetic signals, said process bringing improvements to prior art techniques. Said process also relates to biological analysis consisting in recording the electromagnetic or electrical "signatures" corresponding to known biochemical elements, and to compare such pre-recorded "signatures" to that of a biochemical element to be characterized. Said process implicates filtration and dilution steps in order to eliminate microorganisms and cells present within the original sample, the highest dilutions generating the most electrical or electromagnetic signals whereas the least diluted samples don't provide, most of the time, any electrical or electromagnetic signals. The inventor also showed that microorganisms of different nature, such as bacteria and viruses, produce "nanostructures" that persist in aqueous solutions, and that these very "nanostructures" are emitting electromagnetic signals. Said "nanostructures" behaves like polymers of a size less than 0.02 [mu]m for viruses, and less than 0.1/[mu]m for classic size bacteria, and present a density ranging from 1.12 and 1.30 g/ml.[0005] The process described in this application is based on the astonishing observation that in absence of physical contact, the mere vicinity of a closed tube containing a sample of a bacterial or viral filtrate, little diluted and negative with regard to electrical or electromagnetic emitting signals, inhibits the signals produced by a more diluted sample of the same filtrate, initially positive with regard to electrical or electromagnetic signal emission. In this application, such inhibition will be indistinctly called "inhibitory effect" or "negativing effect". In the same way, in this application, to "inhibit" and "negativate" will be used indistinctly and have a similar meaning. This observation led the inventor to search for the same inhibitory phenomenon from an infected human being. It has been observed, in a patient suffering from an auto-immune microvascularitis of infectious origin, that the diluted samples of his plasma had an inhibitory effect on dilute filtrates of E. coli emitting electromagnetic signals (hereafter EMS), suggesting that the patient was suffering from a chronic infection by this or a related germ. It was also shown that the patient suffering from microvascularitis, as mentioned in the previous example, himself inhibits the EMS emitted by his filtered and diluted plasma, and also inhibits the EMS emitted by a filtered and diluted sample of E. coli culture present in a closed tube. In this case, a 5 minutes contact of a positive dilution in the patient's hand, or 10 minutes at a distance of up to 50 cm, are sufficient to observe said inhibitory effect.[0006] Said inhibitory power thus involves both the emitting structures from one own plasma, and those of a specific bacterial germ, which could thus be used as a universal identification system.[0007] The invention may therefore enable to determine a bacterial or viral origin in illnesses where such germs have not been identified.[0008] A first object of the invention concerns a method for preparing reagents to be used in a test for detecting a microorganism and notably an infection in humans or animals. According to its most general acception, the method includes the following steps:[0000] a) Centrifuging a biological or artificial liquid medium containing a selected specific microorganism;b) Filtrating the supernatant obtained at step (a);c) Preparing a series of diluted samples corresponding to increasing dilutions of the filtrate obtained in step (b), down to a filtrate dilution factor of at least 10;d) Submitting the diluted samples obtained in step (c) to an electrical, magnetic and/or electromagnetic exciting field;e) Analyzing the electrical signals detected using a solenoid and recording digitally aforesaid electrical signal, after analog/digital conversion of aforesaid signal;f) Selecting diluted samples from which the characteristic electrical signals were obtained in (e), by characteristic signals one means signals whose amplitude is at least 1.5 times greater than background noise emitted by water, and/or presenting a frequency displacement towards higher values;g) Introducing the diluted samples selected in step (f) in protective enclosures, which protect said dilutions from very low frequency external electromagnetic fields;h) Distributing one of aforesaid diluted samples from step (g), volume by volume, in two tubes, T1 and T2, with T1 remaining in a protective enclosure protecting said diluted samples from external electromagnetic field interferences, said tube T1 acting as a reference solution, while tube T2, also placed in a protective enclosure, is subsequently being subjected to the presence or contact of a sample suspected of containing said selected specific microorganism.[0009] By "a sample to be tested for presence or absence of aforesaid selected specific microorganism" one means: (i) a human or animal individual suspected to be infected by aforesaid selected specific microorganism, or (ii) a biological specimen or a biological or artificial fluid suspected of containing said selected specific microorganism, or (iii) a food component, a cosmetic, or a pharmaceutical composition susceptible to contain said selected specific microorganism.[0010] By biological fluids, one means any human or animal fluid, e.g. blood, urine, various secretions. By artificial fluid, one means any reconstituted fluid for growing microorganisms, e.g. various culture media for bacteria, yeasts, and molds, and culture media for cells infected by a virus.[0011] Another object of the invention concerns a system for detecting a microorganism within a sample. This system includes:[0000] a) A tube T1 containing a reference sample emitting characteristic electrical signals, by characteristic signals one means signals whose amplitude is at least 1.5 times greater than background noise emitted by water, and/or presenting a frequency displacement towards higher values;b) A tube T2 containing a sample emitting characteristic electromagnetic signal, said sample being identical to that contained in tube T1;c) A protective enclosure for protecting tubes T1 and T2 against very low frequency external electromagnetic fields;d) A tube T3 containing a control solution not presenting electromagnetic signal emission;e) An equipment for receiving electromagnetic signals.[0012] During detection, tube T2 will be subjected to the presence or contact of sample X to be tested for presence or absence of a selected specific microorganism.[0013] Another object of the invention concerns a method for detecting a microorganism within a sample, characterized in that said method consists of the following steps:[0000] a) A sample X, for which the presence of a suspected microorganism, e.g. E. coli, is to be established, is exposed to a sample as obtained after step (f) of the process according to one of claims 1 to 3, said sample obtained after step (f) being a dilution of a culture or biological medium filtrate containing said microorganism suspected to be present in sample X;b) Comparing the electromagnetic signal emitted by sample X exposed to said sample obtained after step (f), obtained in step (a), with the electromagnetic signal emitted by an aliquot of the same sample obtained after step (f) and not submitted to sample X.[0014] By "a sample X", one means (i) a human individual or animal suspected of being infected by aforesaid selected specific microorganism, or (ii) a biological specimen, or a biological or artificial fluid, suspected to contain said selected specific microorganism, or (iii) a food component, cosmetic, or pharmaceutical composition susceptible to contain said selected specific microorganism.[0015] The methods according to the invention enable (i) to prepare reagents intended for a test to detect microorganisms implicated in chronic illnesses, and/or intended to detect systemic latent infections under circumstances where a quick and non invasive response is required, as it is in the case of e.g. avian flu virus detection, (ii) the identification of an infection in humans or animals.[0016] Once the responsible microorganism identified, it is possible to confirm the presence of that germ using supersensitive PCR with specific oligonucleotidic promoters from such microorganism.[0017] The invention shall be better understood by reading the following description, presenting in a non restrictive way examples of process embodiment according to the invention.[0018] The figures in annex correspond to non restrictive examples of embodiment.[0019] An Escherichia coli (E. coli) bacteria culture in LB (Luria broth) medium is centrifuged at 8000 rpm for 15 minutes in order to eliminate the cells. The bacterial supernatant is then filtered on a 0.45 [mu]m porosity PEVD Millipore filter, and the filtrate is then again filtered on a 0.1 [mu]m porosity Millipore filter.[0020] From the resulting E. coli culture filtrate, which is completely sterile, one prepares a series of samples by diluting the filtrate from 10 to 10 into water down to 10for injectable preparation. The successive dilutions are strongly agitated with a vortex for 15 seconds between each dilution.[0021] The diluted samples are distributed in 1.5 ml Eppendorf conic plastic tubes. The fluid volume is in general of 1 milliliter.[0022] Each dilute sample is tested for emission of low frequency electromagnetic signals.[0023] The procedure for detecting EMS includes a step aimed at transforming the electromagnetic field from various diluted samples into one signal, namely an electrical signal, using a solenoid for capturing said electromagnetic field.[0024] The transformation of the electromagnetic field coming from the diluted sample analyzed into an electrical signal is done as follows:[0000] (i) Submitting the dilute sample being checked to an electrical, magnetic and/or electromagnetic exciting field;(ii) Analyzing the electrical signals detected using a solenoid and digitally recording aforesaid electrical signal after analog/digital conversion of said signal;(iii) Selecting the diluted samples generating characteristic electrical signals, by 'characteristic' one means signals whose amplitude is at least 1.5 times greater than background noise signals emitted by water and/or presenting a frequency displacement towards higher values, and placing them in Mumétal(R) protective enclosures for protecting said diluted samples against external electromagnetic field interferences.[0025] Signal detection is carried out using the equipment schematically represented in FIG. 1. The equipment consists of a solenoid reading cell (1) sensitive from 0 to 20000 hertz, placed on a table made of insulating material. Said solenoid used in step (ii) includes a winding comprising a soft iron core. Said winding has an impedance of 300 ohms, an inside diameter of 6 mm, an outside diameter of 16 mm, and a length of 6 mm. The magnetic soft iron core is placed in contact with the external walls of the tube containing the dilution to be analyzed.[0026] The diluted samples to be read are distributed in 1.5 ml Eppendorf (trade mark) conic plastic tubes (2). The fluid volume is in general of 1 milliliter.[0027] Characteristic electrical signal acquisition is performed for a preset duration, i.e. ranging from 1 to 60s. In this example, each sample is read twice successively for 6 seconds.[0028] The electrical signals delivered by the solenoid are amplified and converted into analog-digital signals using a signal acquisition board (sound card) (4) including a computer-built-in analog-to-digital converter (3). Said analog-to-digital converter has twice the sampling rate of the maximal frequency that one wants to digitalize, e.g. 44 kHz.[0029] The digital file corresponding to said converted electrical signal is saved on a mass storage, e.g. as a WAV format audio file.[0030] For processing the characteristic electrical signal, one uses e.g. Matlabs and SigViews (trademarks) software. The recorded digital file may possibly undergo digital processing, i.e. digital amplification for calibrating the signal level, filtering for eliminating undesired frequencies, calculating spectral power distribution (SPD), then such spectral power is truncated, e.g. only keeping frequency bands from 140 Hz to 20 kHz (Matlab), or is transformed in frequency components by Fourier transform (SigView).3) Evaluating the Inhibitory Activity of a Non-Emitting Low Dilution on the Emission of Electromagnetic Signals Generated by an Active Dilution.[0031] The diluted samples presenting characteristic electrical signals are samples diluted to 10, 10, 10. The 10to 10dilutions are negative (FIG. 2).[0032] A closed tube containing a 10dilution aliquot of E. coli is placed side by side with a closed tube containing a 10diluted sample aliquot of E. coli, in an enclosure surrounded by a Mumétal(R) magnetic shield, and left 24 hours at room temperature. In parallel, a control series is realized. This control series consists of one tube containing a 10diluted sample aliquot of E. coli, and of another containing a 10diluted sample aliquot of E. coli that is processed in the same way, but in separate Mumétal(R) enclosures distant from one another. The placement in a Mumétal(R) enclosure eliminates very low active frequencies (5 to 100 Hertz) but not higher frequencies that could come from ambient electromagnetic noise.[0033] After 24 hours, the tubes containing the diluted samples are again analyzed as describes above, revealing that the tube containing a 10diluted sample aliquot and coupled to the tube containing a 10diluted sample aliquot, no longer emits any electromagnetic signals, or much weaker ones. On the other hand, the control series tubes remained identical; the tube containing a 10diluted sample aliquot protected from contact with the tube containing a 10diluted sample aliquot remained positive for electromagnetic signal emission.[0034] An important particularity of the invention is that the observed negating effect is specific, i.e. the lightly diluted, non-emitting sample and the greatly diluted electromagnetic signal-emitting sample must come from the same microorganism species.[0035] Thus, the diluted E. coli-emitting samples are only "negated" by a weakly diluted non-emitting E. coli sample, but not by a lightly diluted non-emitting Streptococcus or Staphylococcus sample. Similarly, a diluted emitting Staphylococcus sample is only "negated" by a lightly diluted non-emitting sample of Staphylococcus and not by a lightly diluted non-emitting sample of Streptococcus or E. coli.[0036] A blood sample, collected with anticoagulant, preferably heparin, from a patient suffering from a neurological pathology consecutive to a bacterial infection, and an Escherichia coli (E. coli) bacteria K1 culture in suspension in LB (Luria broth) medium are centrifuged in order to eliminate the cells. The bacterial supernatant and/or the plasma collected are then diluted to 10in RPMI medium. The solutions are filtered on 0.45[mu] Millipore PEVD filter, then the filtrate is again filtered on 0.02 [mu]m Whatman or 0.1 [mu]m Millipore filter.[0037] From the plasma filtrates of infected individual and from the E. coli K1 culture, one prepares a series of diluted samples corresponding to increasing dilution levels, up to 10, in 10 to 10 dilutions in water for injectable preparation under laminar flow hood. The successive dilutions are strongly agitated with a vortex for 15 seconds between each dilution.[0038] The diluted samples are then distributed in 1.5 ml conic Eppendorf plastic tubes. The fluid volume is in general of 1 milliliter.[0039] The selection of the diluted samples emitting characteristic signals, signals whose amplitude is at least 1.5 times greater than the background noise signals and/or are of a frequency higher than background noise, is realized identically to what is described above in example 1, chapter 2. The method described as well as the material are identical to what is described above. Thus, the method includes a step for transforming the electromagnetic field from different dilutions into a signal, namely an electrical signal, by means of a solenoid capturing said electromagnetic field.[0040] The transformation of the electromagnetic field from the analyzed dilution into an electrical signal is done by:(i) Submitting the diluted sample being checked to an electrical, magnetic and/or electromagnetic exciting field;(ii) Analyzing the electrical signals detected using a solenoid, and digitally recording said electrical signal after analog/digital conversion of aforesaid signal;(iii) Selecting the diluted samples presenting characteristic electrical signals, by 'characteristic' one means signals whose amplitude is at least 1.5 times greater than background noise signals emitted by water, and/or presenting a frequency displacement towards higher values, and placing them in protective enclosures for protecting said diluted samples against external electromagnetic field interferences.[0044] The diluted samples selected at the previous step (item (iii)), from the plasma filtrate of the infected individual, from E. coli culture filtrate, i.e. the dilutions of filtered sample presenting a characteristic electrical signal, are distributed in Eppendorfs plastic tubes, at a rate of 1 ml per tube, and stored at +4[deg.] C. The diluted EMS emitting samples distributed in aliquots are protected from external influences by being placed in an enclosure protected from electromagnetic fields. Preferably, the enclosure is surrounded with a magnetic shield made of Mumétal(R), isolating the enclosure from very low frequency parasitic fields coming from the surroundings.[0045] One of the diluted EMS emitting samples from the plasma filtrate of the infected individual, from E. coli culture filtrate, is distributed volume to volume in two tubes, T1 and T2, with T1 remaining in a protective enclosure protecting said diluted samples from external electromagnetic field interferences, that tube will act as reference solution; tube T2 will be subsequently subjected to the patient and is also placed in a protective enclosure.[0046] Said protective enclosure being preferably surrounded with a Mumétal(R) shield.[0047]represents schematically the steps to take when searching for the inhibitory effect. The search of the inhibitory effect is realized as follows:a) Tube T1, containing the reference solution, remains in an enclosure (3) surrounded by a Mumétal(R) magnetic shield, said tube T1 is thus protected from potential changes of the individual to be examined (4), whereas tube T2 is submitted to the influence of the infected individual to be examined (4) whose plasma present in tubes T1 and T2 comes from, said individual holds T2 in his/her hand (5) for a set period of time, e.g. 5 minutes;b) Tube T2 is placed in an electromagnetic signal reception equipment, preferably a reading solenoid cell as described previously in chapter 2 of this example;c) Electrical signals are then amplified, processed, converted into analog-digital signals as previously described in chapter 2;d) Said analog-digital signals are possibly decomposed in harmonics by Fourrier transform.[0052] The signals corresponding to tube T1 and those corresponding to tube T2, as well as the signals corresponding to water containing tube T3 (background noises) are compared.[0053] The following figures represent the results obtained in the case where the active dilution comes from the examined infected individual plasma:represents a histogram in three dimensions (Matlab) of the electrical signals detected by the solenoid with tube T3 present (background noises);represents a three dimension histogram of the frequency spectrum detected by the solenoid with tube 1 present;represents a three dimension histogram of the frequency spectrum detected by the solenoid with tube 2 present;represents a Fourier analysis (SigView) of the same background noise (the harmonics of the non-filtered current of the power supply);represents a Fourier analysis of the signal detected by the solenoid with tube 1 present;represents a Fourier analysis of the frequency spectrum detected by the solenoid with tube 2 present, handled by the individual to be examined.[0060] The analysis by 3 dimensions histogram, respectively for background noise (FIG. 3) and for the signal obtained with tube T1 present and containing the EMS emitting reference solution (FIG. 4), shows a displacement towards higher frequencies. On the other hand, when analyzing tube T2 containing the solution submitted to the influence of the individual to be examined (FIG. 5), no displacement toward higher frequencies is noted; the 3D histogram representing the signals of tube T2 is analogous to that obtained for background noise.[0061] Fourier analysis of the positive frequencies generated by tube 1 (FIG. 7) revealed peaks at various frequencies. By decreasing order of signal intensity, the following frequencies presented signals: 1000, 2000, 3000, 4100, 5100 and 5500. On the other hand, Fourier analysis of tube T2 reveals results analogous to those obtained by background noise analysis: no significant peak was observed for background noise or for tube T2.[0062] In conclusion, these analyses enable to deduct that the individual examined has a capacity for inhibiting electromagnetic signals emitted by a dilution of his/her own plasma.[0063] Analogous results were obtained with the reference solution, derived from K1 E. coli.[0064] Therefore, this inhibitory capacity concerns not only his/her own plasma but also E. coli emitting structures, suggesting that the individual is infected by an agent producing nanostructures close to those of E. coli.