The non‐obese diabetic (NOD) mouse is a useful animal model for research in human diabetes ( Homann et al ., 1999 ). These mice show signs of insulitis as a result of lymphocytic infiltration of the endocrine part of the pancreas, which leads to decreased production of insulin and increased blood sugar, with its consequent pathologies. In this study, the effect of the oral administration of tobacco chloroplast‐derived proinsulin conjugated to CTB (CTB‐Pins fusion) for the induction of oral tolerance towards insulin was examined. The first report of the accumulation of a valuable therapeutic protein, the CTB‐Pins fusion, in lettuce chloroplasts is also presented.

Clearly, there are advantages to plastid expression; however, in terms of minimally processed orally delivered vegetative biomass, there is a need to move beyond tobacco and to focus on edible crop plant systems. The transformation of plastids in non‐green tissue has been achieved, especially in edible parts of carrot, providing access to several new potential platforms for pharmaceutical production ( Kumar et al ., 2004a , b ; Daniell et al ., 2005b ). For this study, Lactuca sativa (lettuce) was chosen for investigation. Although, recently, two laboratories have reported stable plastid transformation in lettuce, the expression of therapeutic proteins has been unsuccessful ( Lelivelt et al ., 2005 ; Kanamoto et al ., 2006 ).

The oral delivery of biopharmaceutical proteins expressed in plant cells should reduce the costs associated with purification, processing, cold storage, transportation and delivery. However, poor intestinal absorption of intact proteins has been a major challenge. To overcome this limitation, we investigated the concept of receptor‐mediated oral delivery of transgenic proteins ( Limaye et al ., 2006 ). The B subunit of the toxin from Vibrio cholerae (CTB) is recognized as one of the most potent mucosal adjuvants ( Holmgren et al ., 2005 ). CTB and green fluorescent protein (CTB‐GFP), separated by a furin cleavage site, were expressed via the tobacco chloroplast genome. Following the oral administration of CTB‐GFP‐expressing leaf material to mice, GFP was observed in the mice intestinal mucosa, liver and spleen in fluorescence and immunohistochemical studies, whereas CTB remained in the intestinal cell ( Limaye et al ., 2006 ). This report of receptor‐mediated oral delivery of a foreign protein into the circulatory system brings the oral delivery of human therapeutic proteins one step closer to realization.

Diabetes is a disease in which the body does not produce or properly utilize insulin. Type 1 diabetes results from the autoimmune destruction of insulin‐producing cells. The major destruction of β‐cells occurs predominantly from autoreactive T‐cytotoxic cells ( Nagata et al ., 1994 ) and T‐helper‐1 (Th1) cells ( Ploix et al ., 1999 ) reactive to β‐cell autoantigens, such as insulin. In 2002, the American Diabetes Association estimated that 18.2 million people in the USA, or 6.3% of the total population, had diabetes, with more than $120 billion in treatment costs each year. In 2002, diabetes was the sixth leading cause of death in the USA, contributing to 213 062 deaths. The only currently accepted form of treatment is the administration of recombinant insulin, which serves to temporarily replace the missing insulin in diabetic patients. Therefore, it is essential to find a prevention and cure for this debilitating disease.

Blood and urine glucose levels of the treated NOD mice were measured twice, at weeks 6 and 7 of treatment (11‐ and 12‐week‐old mice). The blood glucose values of all groups in the study at both time points tested were below 200 mg/dL, and therefore were not considered as diabetic. This was not unforeseen, as NOD mice typically do not develop high blood glucose until 12–15 weeks of age ( Arakawa et al ., 1998 ). Although, at week 11, the CTB‐Pins‐treated group showed a blood glucose level as high as that of the control animals, interestingly, at week 12, the CTB‐Pins‐treated animals showed a significantly lower blood glucose level than that of the control groups. Urine glucose values were also lower in the CTB‐Pins‐treated group ( Figure 8b ).

Determination of immunoglobulin (Ig) and glucose levels. (a) Serum levels of IgA, IgG2a and IgG1 in non‐obese diabetic (NOD) mice receiving cholera toxin B subunit–human proinsulin (CTB‐Pins)‐expressing plant leaf material. Control groups receiving untransformed plant material (Un‐Tr) or interferon–green fluorescent protein (IFN‐GFP)‐expressing leaf material are also shown. (b) Blood and urine glucose levels in various groups of NOD mice after oral administration of CTB‐Pins (6 weeks post‐treatment). Un‐Tr, n = 1; IFN‐GFP, n = 1; CTB‐GFP, n = 2; CTB‐Pins, n = 2. Using Student's t ‐test, P value is less than 0.05. Bars, standard deviation. n indicates the number of animals in each treatment group.

Serum and intestinal mucosal Ig levels were determined by ELISA using CTB as the capture antigen. Serum levels of IgG1 increased in NOD mice treated with CTB‐Pins‐expressing plant leaf material, relative to the control groups. Low serum IgG2a and mucosal IgA levels against CTB were observed in NOD mice treated with untransformed plant leaf material or plants expressing IFN‐GFP or CTB‐Pins ( Figure 8a ).

Immunostaining for cytokine production. (a) Interleukin‐10 (IL‐10) immunoreactivity in the pancreas of three mice administered untransformed plant leaf material (i–iii). Blood vessels (BV) and Langerhans islets (isl) are indicated. (iv–vi) Islets of mice receiving cholera toxin B subunit–human proinsulin (CTB‐Pins). Small arrows indicate perivascular infiltration of IL‐10‐expressing lymphocytes. Large arrows indicate IL‐10‐positive lymphocytes inside or around the islets. (b) Interleukin‐4 (IL‐4) immunoreactivity in the pancreas of mice receiving interferon–green fluorescent protein (IFN‐GFP), CTB‐GFP or CTB‐Pins plant leaf material. Small arrows indicate position of the islets.

Oral administration of CTB‐Pins to NOD mice led to an increased recruitment of immunosuppressive cytokine‐producing cells (lymphocytes) to the pancreas. A large number of interleukin‐4 (IL‐4) and interleukin‐10 (IL‐10)‐producing cells were seen proximal to the pancreatic islets, which were recruited through the circulation. This process was supported by significant perivascular migration of IL‐4‐ and IL‐10‐expressing cells in the pancreases of CTB‐Pins‐treated NOD mice ( Figure 7a,b ).

Assessment of insulin production and apoptosis in pancreatic β‐cells. (a) Insulin immunoreactivity in Langerhans islets of a mouse receiving cholera toxin B subunit–human proinsulin (CTB‐Pins). (b) Caspase‐3 immunostaining in the same section is shown in the red channel. (c) Merged picture of (a) and (b). (d) A view of the pancreas showing the remnant of a large Langerhans islet in a mouse receiving untransformed plant leaf material. (e) Caspase‐3 immunoreactivity in the same section taken in the red channel. (f) Merged picture of (d) and (e).

We next determined whether the remaining β‐cells in the pancreases of the different treatment groups were apoptotic. Because cellular infiltration can lead to apoptosis, this can be used as a hallmark to study type 1 diabetes ( Riedl and Shi, 2004 ). It was found that the β‐cells from NOD mice treated with CTB‐Pins rarely expressed caspase‐3, suggesting that apoptosis was prevented in these cells. In the other experimental groups, even the very few remaining insulin‐producing β‐cells expressed activated caspase‐3, suggesting that they were undergoing apoptosis ( Figure 6 ).

(a) Histochemical staining of pancreatic sections. (i) Haematoxylin and eosin staining of a section of the pancreas (showing an islet, isl) of a mouse receiving cholera toxin B subunit–human proinsulin (CTB‐Pins) for 7 weeks ( n = 7); scale bar, 50 µm. Lymphocytes are seen outside the islet (arrow). (ii) Arrows indicate the borders of an islet in the pancreas of a mouse receiving CTB–green fluorescent protein (CTB‐GFP) ( n = 5; control group). Blue dots show lymphocytic infiltration of the islet. (iii) A large islet with severe lymphocytic infiltration in a mouse receiving untransformed plant leaf material (UN‐Tr; n = 3). (iv) Severe lymphocytic infiltration in a mouse receiving interferon–GFP (IFN‐GFP) ( n = 5). (b) Scoring (S) of the degree of insulitis according to the severity of the lymphocytic infiltration of the pancreatic Langerhans islets. Score 1, no or pre‐islet infiltration; 2, minimal infiltration; 3, moderate infiltration; 4, severe infiltration; 5, more than 80% of the islets infiltrated. All sections were scored in a blind manner. (c) Graphic representation of insulitis scoring in untransformed, IFN‐GFP, CTB‐GFP and CTB‐Pins plant‐treated groups; bars represent standard deviation (* P < 0.05). n indicates the number of animals in each treatment group.

To quantify and compare insulitis between the treatment groups, representative sections were prepared and cellular infiltration was scored in a blind manner. Fifty sections per animal were analysed. The average score indicated that the pancreases from NOD mice treated with CTB‐Pins showed minimal cellular infiltration, and this cellular infiltration was significantly less than in all the other treatment groups ( Figure 5a–c ).

Insulitis is characterized by lymphocytic infiltration of the pancreatic islets, which leads to their destruction, including the insulin‐producing β‐cells. The pancreases were collected from 12‐week‐old NOD mice from the different treatment groups to assess the degree of insulitis.

Despite a number of experimental approaches, we were unable to establish the expression level of CTB‐Pins in tobacco or lettuce plants via enzyme‐linked immunosorbent assay (ELISA). The highest absorbance values were observed in the GM 1 binding assay from samples extracted under reducing conditions. Although we would expect reduction of disulphide bonds to abrogate the ability of our fusion protein to associate with the plate‐bound receptor in pentameric form ( Ludwig et al ., 1985 ; Dertzbaugh and Cox, 1998 ), plant extracts prepared in western extraction buffer [14 mm (beta)‐mercaptoethanol (β‐me)] or with a molar excess of dithiothreitol (0.5 m DTT) clearly facilitated GM 1 binding, as indicated by elevated absorbance readings. The potential for protein aggregation to occur in plant extracts increases with the concentration of the protein in question. Together, CTB monomers and the proinsulin molecule contain several cysteine residues through which disulphide bonds form, both intramolecularly and intermolecularly. We believe that the aggregation of the CTB‐Pins fusion confounded our efforts to execute quantitative ELISAs.

Protein analyses. Western blots prepared from wild‐type (WT) and transplastomic lettuce and tobacco were probed with human proinsulin monoclonal antibody. (a) Total protein (~20 µg) extracted from lettuce leaves was loaded into wells for each sample. In lane 6, L101‐5, ~10 µg of total soluble protein (TSP) was loaded. (b) Total protein (~10 µg) extracted from tobacco leaves was loaded into wells. (c) Cholera toxin B subunit–human proinsulin (CTB‐Pins) in plant samples was detected by polyclonal anti‐CTB and quantified by comparison with known quantities of CTB standard. Lanes 1–3, bacterial CTB (25, 50, 100 ng). Lanes 4–6, transplastomic tobacco lines 5CP‐13, 5CP‐14, 5CP‐M (~6 µg of TSP in each lane). Lanes 7 and 8, transplastomic lettuce lines L‐100 and L‐101 (~36 µg TSP in each lane). (d) Plot of integrated density values (IDVs) for quantitative analysis from standard curve. Broken line, data points; full line, trend line. (e) Estimation of CTB‐Pins in tobacco and lettuce leaves using spot densitometry CTB immunoblots. (f) Tobacco and lettuce transformants were assayed for GM 1 binding. 5CP, CTB‐Pins tobacco; L101 and L101, CTB‐Pins lettuce; BSA, negative control (bovine serum albumin).

Immunoblots probed with the human proinsulin monoclonal antibody showed the presence of an ~22‐kDa fusion protein in the chloroplast transgenic lines. The formation of dimers, trimers, tetramers and pentamers of the CTB‐Pins fusion protein was also observed ( Figure 4a,b ). A similar banding pattern was observed by immunodetection with CTB polyclonal antibody ( Figure 4c ). Quantification of the fusion protein on western blots was performed by comparing plant samples with known quantities of purified CTB and analysing them by spot densitometry. Linearity of the standard curve was achieved using 25, 50 and 100 ng of CTB, facilitating the estimation of CTB expression in samples in the same blot ( Figure 4d ). The three tobacco transgenic lines were found to contain up to 178.2, 126.7 and 139.1 µg of CTB‐Pins per 100 mg of leaf tissue, i.e. approximately 16% of total soluble protein (TSP) ( Figure 4e ). Such variation could be the result of the use of fresh vs. frozen plant material for these assays, or differences in sample preparation or growth conditions. Lettuce lines L100 and L101 accumulated up to 13.6 and 15.3 µg per 100 mg of leaf tissue, respectively, approximately 2.02% and 2.43% of TSP. The GM 1 binding assay demonstrated that pentameric structures of CTB‐Pins were formed ( Figure 4f ). This assay confirmed the correct folding and disulphide bond formation of CTB pentamers within transgenic chloroplasts, as only the pentameric structure of CTB has the ability to bind to the GM 1 receptor ( Merritt et al ., 1994 ).

For the confirmation of homoplasmy in lettuce transgenic lines, labelled flanking sequence probe (1.3 kb) was hybridized to Bgl II‐digested genomic DNA. The hybridization pattern showed only the expected 3.75‐kb fragment in the WT sample and only the expected 6.15‐kb fragment in lettuce transformants after second regeneration ( Figure 2c ). Southern blotting was also carried out with genomic DNA samples from the primary regenerants. Although the L100 line demonstrated heteroplasmy, with both WT and transformed fragments hybridizing with the probe, primary regenerant L101 appeared to be homoplasmic (data not shown). Previous studies with tobacco have demonstrated that homoplasmy can indeed be achieved in the first round of selection ( Guda et al ., 2000 ), because the flanking sequence contained an origin of replication (thereby providing more templates for integration). As the lettuce transformation vector includes full‐length lettuce trn I gene, which probably contains Ori A, it is not unreasonable to find this phenomenon in lettuce plastid transformants as well.

Chloroplast transgenic lines were examined by Southern analysis in order to confirm site‐specific integration and to determine whether they were homoplasmic or heteroplasmic. Homoplasmy is achieved when all the copies of the genome within the chloroplast have stably integrated transgenes. For tobacco, the gene‐specific probe ( CTB‐Pins ) taken from the pLD‐5CP vector by Mfe I/ Not I digestion hybridized to a single 6.4‐kb fragment in transgenics, but not to any WT plant DNA fragment (data not shown). The flanking sequence probe contained regions of the trn I and trn A genes. In most of the transgenic lines, only the 6.4‐kb fragment was seen when hybridized with this probe ( Figure 1b ), indicating that homoplasmy was achieved within limits of detection by Southern blot.

Production of transplastomic Latuca sativa and confirmation of maternal inheritance. (a) Lettuce plants propagated by rooting of nodal cuttings were transferred to soil in the glasshouse. Plants matured with no apparent aberrant phenotype (b) and produced normal inflorescences (c). Flowers heads opened (d), and seeds were harvested. T 1 seeds were plated on half‐strength Murashige and Skoog (MS) medium containing 50 mg/L spectinomycin, together with wild‐type seed (e). T 1 plants flourished and were transferred to the glasshouse (f).

The bombardment of 60 lettuce leaves resulted in two independent transformation events (lines L100 and L101), identified as green shoots arising directly from completely bleached tissue on lettuce regeneration (LR) medium containing 50 mg/L spectinomycin ( Figure 2d ). It should be noted that no callus was formed prior to the initiation of shoots from leaf explants. Following an additional round of selective regeneration, a progenitor for each line was rooted in MS medium containing spectinomycin (50 mg/L) and multiplied by clonal propagation. Clones were transferred to soil ( Figure 3a ) and moved to the glasshouse, where they matured ( Figure 3b ), bolted and produced normal panicles ( Figure 3c ) and inflorescences with disc flowers ( Figure 3d ). Pappus‐bearing achenes (seeds) were harvested. Lettuce seeds (T 1 ) were sterilized and germinated on spectinomycin‐containing medium (50 mg/L) together with wild‐type (WT) seeds ( Figure 3e ). T 1 seeds germinated and grew into uniformly green plants ( Figure 3f ). The absence of Mendelian segregation of transgenes indicated that they were maternally inherited to progeny. Most WT seeds failed to germinate on spectinomycin‐containing medium. Of the 30 WT seeds plated, six reached radicle emergence, but hypocotyl emergence was not observed and none developed into seedlings.

The bombardment of 10 tobacco leaves resulted in 56 independent transformation events, 40 of which were subjected to three rounds of selection, two on regeneration medium of plants (RMOP) and one on Murashige and Skoog medium without hormones (MS0) medium containing 500 mg/L spectinomycin. Integration of the transgene cassette was confirmed by polymerase chain reaction (PCR).

Regeneration and Southern analysis of cholera toxin B subunit–human proinsulin (CTB‐Pins) lettuce transformants. (a, b) Schematic diagrams of lettuce transformation vector and integration cassette, integration site and resulting transplastome. Full lines indicate the sizes of the integration cassette (2.4 kb) and expected fragments for the wild‐type (3.75 kb) and transformed (6.15 kb) genomes in Southern analysis; broken line indicates the probe hybridization sites. (c) Southern analysis of second regenerants. L100 and L101, independent transplastomic lines; WT, wild‐type. (d) Primary regeneration in lettuce without formation of callus.

The L. sativa long flanking plastid transformation vector (pLS‐LF, Figure 2a ) was constructed using primers derived from regions of known conservation in the Nicotiana tabacum plastome to amplify cognate sequences from the L. sativa plastome. The full‐length genes for plastid trnl (Ile) (1020 bp) and trnA (Ala) (887 bp) were amplified and cloned. The unique Pvu II site was used to insert transformation cassettes into the intergenic spacer region between the tRNAs. Long flanking sequences encoding portions of the 16S (810 bp) and 23S (974 bp) ribosomal RNA subunits were included to enhance homologous recombination between the vector and the host plastome. The tobacco native plastid ribosomal operon promoter (P rrn ) and 3′ UTRs ( psbA and rps 16) were used to drive the expression of AadA from the GGAGG ribosome binding site and CTB‐Pins from the 5′‐translation control element of bacteriophage T7 gene10 ( Figure 2a ). Following the assembly of pLS‐LF‐CTB‐Pins, plasmids were isolated from spectinomycin‐resistant cultures and correct orientation was confirmed by Sac I digest.

Five‐week‐old mice were used in this study to demonstrate the alleviation of symptomatic pancreatic insulitis and the preservation of insulin‐producing β‐cells, a condition that mimics human type 1 diabetes. Based on the success of the concept in older mice ( Harrison et al ., 1996 ), this strategy is likely to work not only prior to the onset of diabetes, but also at later stages of this autoimmune disease, and this will be explored in future experiments. One previous human clinical study on the oral delivery of insulin was unsuccessful ( Skyler et al ., 2005 ), because insulin was not protected from digestive enzymes and acid hydrolysis. In our study, however, insulin was protected by bioencapsulation within plant cells. On the basis of the results obtained in this study, human clinical trials have been initiated.

Taken together, the data presented here suggest that the suppression of insulitis is mediated by regulatory Th2 cells. As T‐cell regulation plays a major role in mucosal immunity, the oral administration of an autoantigen can be used to treat autoimmune diseases in animal models by generating active T‐cell suppression. Several autoimmune diseases and their antigens are known: multiple sclerosis (myelin basic protein and proteolipid protein), arthritis (type II collagen), uveitis (S‐antigen and interphotoreceptor retinoid binding protein), myasthenia gravis (acetylcholine receptor) and thyroiditis (thyroglobin) ( Hafler and Weiner, 1997 ). In the USA, 5.5 million people suffer from psoriasis, 3 million from Graves’ disease, 2.5 million from rheumatoid arthritis, 2–5 million from vitiligo, 3.5 million from thyroiditis, 1–4 million from Sjogren's syndrome, 0.5 million from Crohn's disease and multiple sclerosis, 370 000 from type 1 diabetes, etc. This study opens up the possibility for new investigations on autoimmune diseases.

The oral administration of self‐antigens, such as insulin, leads to their uptake by gut‐associated lymphoid tissue (GALT), including intestinal mucosal M‐cells, which pass the antigen to underlying antigen‐presenting cells ( Limaye et al ., 2006 ). This leads to the activation of T‐cells and the induction of a Th2 cell response, which is characterized by the up‐regulation of immunosuppressive cytokines (such as IL‐10 and IL‐4) and serum antibodies (such as IgG1, but not IgG2a) ( Salmond et al ., 2002 ; Faria and Weiner, 2005 ). No significant increase in mucosal IgA was seen in our study in CTB‐Pins‐treated mice vs. the control groups. CTB‐Pins‐treated animals showed very high levels of IgG1, but not IgG2a, whereas the control groups showed no variation ( Figure 8a ). The serum IgG1 values of CTB‐Pins‐treated animals confirm the activated Th2 response, which is also supported by the histology, with less lymphocytic infiltration, the up‐regulation of immunosuppressive cytokine levels in the tissues, and the trend in the blood and urine glucose levels (which were higher in the control groups than in the CTB‐Pins‐treated group). The presence of CTB in the intestine ensures effective receptor‐mediated oral delivery of intact plant‐derived fusion protein across the intestinal mucosa via the binding of CTB to the GM 1 ganglioside receptor and uptake by intestinal M‐cells and enterocytes.

Although lower levels of CTB‐Pins accumulation were observed in transplastomic lettuce when compared with tobacco (approximately sixfold less in lettuce), the average value determined for lettuce (~1.8% of TSP) represents a level of protein sufficient to proceed with animal or preclinical studies. For example, in this study, using tobacco, we delivered approximately 14 µg of CTB‐Pins to NOD mice; a comparable dose could be derived from 100 mg of fresh lettuce leaf, a feasible quantity for weekly oral delivery. The difference observed between tobacco and lettuce may be attributed, in part, to the 5′ regulatory elements used in our study. Tobacco expression of CTB‐Pins is driven by the endogenous psbA 5′ UTR, whereas lettuce expression is regulated by the inclusion of the translational control region of bacteriophage T7 gene 10. Previous studies have demonstrated that the level of foreign protein accumulation is lower when these translation elements are used to drive expression of the same gene, with psbA 5′ UTR being more efficient ( Dhingra et al ., 2004 ). In addition, intrinsic variation in the nature of the leaves from tobacco and lettuce may influence the accumulation of foreign protein expressed in chloroplasts. We are developing new transformation constructs for lettuce for CTB‐Pins expression which will employ lettuce endogenous translation elements, such as psbA 5′ UTR, to further increase the level of expression.

Previous studies expressing the CTB‐Pins fusion protein in plants have been performed in potato ( Arakawa et al ., 1998 ). The expression level in nuclear transgenic potato tubers was 0.1% of TSP. This low expression level required the feeding of NOD mice with large amounts of fresh potatoes. In the present study, the CTB‐Pins fusion protein accumulated in transplastomic tobacco to up to ~16% of TSP, 160‐fold greater than that achieved in nuclear transgenic potatoes. NOD mice were given 8 mg of CTB‐Pins tobacco leaf tissue (containing ~14 µg of the fusion protein) per week by gavage; this represents a 375‐fold decrease in the amount of plant tissue administered compared with the 3 g per week used previously ( Arakawa et al ., 1998 ). The use of these small concentrated doses reduces the possibility of the potential confounding effects of leaf tissue, and eliminates the need to process or purify large quantities of plant material. Hyper‐expression of CTB‐Pins in plant plastids should make this fusion protein abundantly available for animal studies or human clinical trials.

Experimental procedures

Vector construction The human proinsulin gene was synthesized according to Prodromou and Pearl (1992). The PCR product was then cloned into the PCR 2.1 vector and the sequence was verified. The psbA promoter and 5′ UTR were amplified from the tobacco chloroplast genome, followed by subcloning and sequence verification. The promoter‐5′UTR fragment was then spliced together with CTB and human proinsulin by overlap extension (Horton et al., 1989). The construct containing 5′UTR‐CTB, a GPGP hinge region (introduced by mutagenesis to allow for the correct folding of each protein by reducing steric hindrance) and human proinsulin was designated as 5CP. Following SalI/NotI digestion, the fusion gene was ligated into the pLD‐ctv chloroplast transformation vector (Daniell et al., 1998, 2004b). The pUC‐based L. sativa long flanking plasmid (pLS‐LF; Figure 2a) was constructed to integrate foreign genes into the intergenic spacer region between the trnI (Ile) and trnA (Ala) genes of the plastid genome inverted repeat region. Oligonucleotide primers were derived from regions of known conservation in the N. tabacum plastome, and carried end modifications for restriction enzyme sites for use in vector assembly. The full‐length genes for plastid trnl (Ile) (position 101 979–102 998) and trnA (Ala) (position 103 063–103 949) were amplified and ligated into the pUC19 backbone. A unique PvuII recognition site (position 103 002) between the two sequences facilitated the insertion of transformation cassettes. Long flanking sequences encoding the 3′ end of the 16S (100 876–101 979; 810 bp) and 5′ end of the 23S (104 102–105 075; 974 bp) ribosomal RNA subunits were amplified and cloned in kind. The numeric values correspond to the positions in the L. sativa plastome (NC_007578). The transformation cassette (Figure 2a) was assembled in pZERO (Invitrogen, Carlsbad, CA, USA) and included the following published tobacco plastid regulatory sequence elements: ribosomal operon promoter (Prrn), rps16 and psbA‐3′ UTRs. The 5′ translation control region of bacteriophage T7 gene 10 was used to drive CTB‐Pins expression and the aadA gene was included with a GGAGG ribosome binding site. The expression cassette was flanked with SnaB1 recognition sites. The PvuII‐digested pLS‐LF was treated with alkaline phosphatase prior to ligation with the SnaB1‐digested cassette. The recovered plasmids were digested with SacI to determine the correct orientation of the inserted cassette in pLS‐LF. All cloning steps were carried out in Escherichia coli according to the methods of Sambrook and Russel (2001).

Bombardment and selection of transgenic plants The bombardment and regeneration of N. tabacum cv. Petit Havana transformants were carried out as described previously (Kumar and Daniell, 2004). Seeds of L. sativa v. Simpson elite (New England Seed Co., Hartford, CT, USA) were surface sterilized in a 3% hypochlorite solution, rinsed three times in water and plated on Murashige and Skoog (MS) medium solidified with 5.8 g/L Phytablend® (Caisson, North Logan, UT, USA). Young, fully expanded leaves (~4 cm2) were placed, adaxial side up, on antibiotic‐free LR medium (Kanamoto et al., 2006). The leaves were bombarded with 0.6‐µm gold particles (Bio‐Rad, Hercules, CA, USA) coated with pLS‐LF‐CTB‐Pins (Figure 2a), as described by Kumar and Daniell (2004), employing 900 psi rupture discs and a target distance of 6 cm. Samples were held in the dark at 25 °C for 2 days prior to the explan of 0.5‐cm2 pieces, adaxial side down, on to LR medium containing 50 mg/L spectinomycin dihydrochloride. Primary regenerants were screened by PCR for the transplastomic event, and positive shoots were subjected to an additional regeneration cycle on LR medium containing spectinomycin. Following the second regeneration, the shoots were rooted in half‐strength MS medium containing 0.1 mg/L naphthaleneacetic acid (NAA) and 50 mg/L spectinomycin. The plants were propagated by the rooting of nodal sections in half‐strength, hormone‐free MS medium containing spectinomycin. Rooted cuttings were hardened in Jiffy® peat pots before transfer to the glasshouse for seed production. T 1 seeds (achene) were harvested when the pappus was present, and allowed to dry at 24 °C. Sterile seeds (100) were plated on MS medium containing 50 mg/L spectinomycin.

Southern blot analysis Southern blot analysis was carried out essentially according to Kumar and Daniell (2004). Total tobacco DNA was digested with AflIII, separated on a 0.7% agarose gel at 45 V for 4 h, and then transferred to a nylon membrane. The pUC‐CT vector DNA was digested with BamHI and BglII to generate a 0.8‐kb probe, which was used as a flanking probe, and pLD‐CTB‐Pins was digested with MfeI and NotI to generate a 0.36‐kb gene‐specific probe. After labelling the probe with 32P, hybridization of the membranes was performed using the QUICK‐HYB hybridization solution and protocol (Stratagene, La Jolla, CA, USA). For lettuce transformants, genomic DNA was digested to completion with BglII, separated on 0.7% Tris‐acetate‐EDTA (TAE)‐agarose and transferred to nylon membranes. The plastid flanking sequence probe (1.3 kb) was amplified by PCR from lettuce genomic DNA. The PCR product was purified, and labelled probe was generated by incubation with 32P and Ready‐To‐Go™ DNA Labelling Beads (‐dCTP) (GE Healthcare, El Paso, TX, USA). Hybridization was carried out at 68 °C with washing at 37 °C and 60 °C. Radiolabelled blots were exposed to film at –80 °C for 16 h.

Western blot and densitometric analysis TSP was isolated from rooted second regenerants of tobacco and lettuce. TSP from approximately 100 mg of leaf tissue (10 or 20 micrograms) was separated by sodium dodecylsulphate‐polyacrylamide gel electrophoresis (SDS‐PAGE) and transferred to nitrocellulose membranes for immunoblotting, according to Kumar and Daniell (2004). Anti‐proinsulin monoclonal antibody (American Qualex, 1 : 20 000, San Clemente, CA, USA) and goat anti‐mouse IgG conjugated to horseradish peroxidase (HRP) (American Qualex, 1 : 15 000) were used for the detection of the CTB‐Pins protein. Immunoblotting with anti‐CTB primary antibody (1 : 4000, Sigma, St. Louis, MO, USA) and HRP‐conjugated donkey anti‐rabbit secondary antibody (1 : 12 500, Biomeda, Foster City, CA, USA) was employed for spot densitometric analysis. For transplastomic lettuce samples, 36 µg of TSP was added to each well; for transplastomic tobacco samples, 6 µg of TSP was added to each well. The standards (CTB; Sigma) contained 25, 50 and 100 ng of purified bacterial CTB. A SuperSignal® West Pico HRP Substrate Kit (Pierce, Rockford, IL, USA) was used for autoradiographic detection. Following exposure to film, the blots were analysed for the presence of CTB‐Pins using AlphaImager® and AlphaEase® FC software (Alpha Innotech, San Leandro, CA, USA), by comparison with known quantities of standard.

GM 1 binding assay In order to test the ability of chloroplast‐derived CTB‐Pins to bind to the GM 1 receptor, a CTB–GM 1 binding assay was performed. Tobacco extracts were prepared in ELISA buffer and lettuce extracts were prepared in western extraction buffer. Ninety‐six‐well plates were incubated with monosialoganglioside‐GM 1 (Sigma) (3.0 µg/mL in bicarbonate buffer) and bovine serum albumin (BSA) as a control, and incubated overnight at 4 °C. Following washing [three times each with 1X phosphate buffered saline with 0.05% (v/v) Tween 20 (PBST) and sterile water], the plate was blocked with 1X PBST (0.1% Tween 20) with 3% dry, non‐fat milk (PTM) (tobacco) or 0.25% BSA in phosphate‐buffered saline (PBS) (lettuce) for 1 h at 37 °C. CTB standards (Sigma) and soluble protein extracts were diluted in ELISA plant extraction buffer [without Tween‐20 and phenyl methyl sulphonyl fluoride (PMSF)]. The standards and samples were then added in duplicate and incubated at 4 °C overnight. Rabbit anti‐CTB primary antibody (1 : 8000 tobacco, 1 : 3000 lettuce; Sigma) and HRP‐conjugated donkey anti‐rabbit secondary antibody (1 : 25 000 tobacco and 1 : 12 500 lettuce; Biomeda) were used to detect the binding of CTB‐Pins to the GM 1 receptor. The plate was washed thrice with both PBST and sterile water, and 100 µL of tetra‐methyl benzidine (TMB) soluble solution substrate (American Qualex) was added to the wells and incubated in the dark for 30 min. The reaction was stopped with 50 µL of 2 m H 2 SO 4 , and read on a plate reader (Dynex Technologies, Chantilly, VA, USA) at 450 nm.

Animal studies Four‐week‐old, female, NOD mice were purchased from The Jackson Laboratory (Bar Harbor, ME, USA). Mice were kept in the UCF Wild Animal Facility under normal light/dark cycle conditions and had access to food and water ad libitum. The oral administration of CTB‐Pins‐expressing transgenic tobacco or control plant leaf material began when the animals were 5 weeks of age, to allow the mice 1 week to acclimatize to the facility. The mice were divided into the following groups: group 1 received untransformed plant leaf material (Un‐Tr); group 2 received transgenic plant leaf expressing CTB conjugated to GFP (CTB‐GFP); group 3 received transgenic plant leaf expressing IFN conjugated to GFP (IFN‐GFP); and group 4 received CTB‐Pins‐expressing transgenic plant leaf. Each group contained five animals, except for the CTB‐Pins group, which contained seven. The mice were given 14 µg of the specified ground tobacco leaf material diluted in 200 µL of PBS (0.1 m) by careful gavage into the hypopharynx once a week for 7 weeks. For preparation of the gavage material, leaves were frozen and ground in liquid nitrogen. For oral delivery, 8 mg of the CTB‐Pins‐expressing plant leaf material contained 14 µg of the CTB‐Pins protein. For the untransformed leaf material, 8 mg of the ground plant material was given to mimic a similar oral dose to the CTB‐Pins group. The CTB‐GFP and IFN‐GFP levels were similar to that of CTB‐Pins. The animals were sacrificed at 12 weeks of age, the pancreas and other tissues were collected, and both blood and urine glucose levels were measured.

Histochemistry for lymphocytic infiltration and insulitis Following the 7 weeks of treatment, the mice were sacrificed and perfused transcardially with 10 mL of PBS, followed by 50 mL of 4% paraformaldehyde (PFA) in 0.1 m PBS. Part of the pancreas was saved before fixation and freshly frozen in Tissue Tec freezing medium (Vector Laboratories, Burlingame, CA, USA). The remaining pancreas was removed, postfixed overnight in 4% PFA, and cryo‐protected by serially passing through 10%, 20% and 30% sucrose solutions in PBS. The pancreatic tissue was then immersed in Tissue Tec freezing medium and frozen (Samsam et al., 2003) in liquid nitrogen‐cooled isomethylbutane (isopathane, Sigma). Frozen sections of the pancreas, 10 µm thick, were prepared using a cryostat. Pancreas cryosections were stained with haematoxylin and eosin, dehydrated in serial graded alcohol solutions, and the slides were covered. Insulitis levels were measured using the extent of lymphocyte infiltration of the islets of Langerhans. At least 50 sections per animal were scored. The degree of insulitis was scored on a scale of 1–5, where score 1 denotes a normal islet with no sign of T‐cell infiltration, and score 5 indicates maximal infiltration and the development of insulitis.

Immunohistochemistry for insulin, caspase‐3, IL‐4 and IL‐10 Immunohistochemistry for the localization of insulin, caspase‐3 (a final molecule of apoptosis) and the immunosuppressive cytokines IL‐4 and IL‐10 was performed on pancreas cryosections. Sections were blocked with 10% BSA containing 0.3% Triton‐X100. Polyclonal guinea pig anti‐insulin, polyclonal rabbit anticaspase‐3, and rat monoclonal anti‐IL‐4 and anti‐IL‐10 primary antibodies (Invitrogen) were diluted at a concentration of 1 : 300 in 1% BSA in PBS containing 0.3% Triton‐X. Fluorescent conjugated secondary antibodies were goat anti‐guinea pig Alexa Fluor 488 (green), goat anti‐rabbit Alexa Fluor 555 (red) and goat anti‐rat Alexa Fluor 555 (red; Invitrogen).

Antibody titre Serum and intestinal antibodies were assayed for the presence of anti‐CTB antibodies using colorimetric ELISA methods. Following sacrifice and prior to transcardial perfusion, 200–300 µL of blood was collected from the retro‐bulbar vein. Serum was extracted after 15 min of centrifugation at 3000 × g at 4 °C for antibody titre. Ninety‐six‐well plates were coated with CTB (Sigma). Serial dilutions of serum or supernatants of faecal pellets (five pellets per sample were weighed and diluted in 0.1 m PBS), collected from the different animal groups, were added to the coated plate wells. For standard values (isotype control) and determination of antibody level, the standard columns of the plate were coated with serial dilutions of purified mouse IgG1 or IgG2a, or IgA protein (BD Pharmingen, Franklin Lakes, NJ, USA), and ELISA was performed. Secondary antibodies were HRP‐conjugated anti‐mouse IgG2a, IgG1 and IgA antibodies (BD Pharmingen) at a concentration of 1 : 3000 in PBS containing 0.1% Tween‐20 and 3% milk powder. The plates were washed with 200 µL of PBS, and the substrate TMB was added to the wells and incubated in the dark at 37 °C for 20 min. The reaction was stopped by adding 50 µL of H 2 SO 4 , and the plates were read on a plate reader (Dynex Technologies) at 450 nm.