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Peptide-Mediated Targeting of the Islets of Langerhans

¹ Center for Biomedical Inventions, Department of Internal Medicine, University of Texas Southwestern Medical Center, Dallas, Texas
² Sarah W. Stedman Nutrition and Metabolism Center, Departments of Pharmacology and Cancer Biology, Medicine, and Biochemistry, Duke University Medical Center, Durham, North Carolina

	ABSTRACT

TOP ABSTRACT RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

 
Strategies for restoring ß-cell function in diabetic patients would be greatly aided by the ability to target genes, proteins, or small molecules specifically to these cells. Furthermore, the ability to direct imaging agents specifically to ß-cells would facilitate diagnosis and monitoring of disease progression. To isolate ligands that can home to ß-cells in vivo, we have panned a random phage-displayed 20-mer peptide library on freshly isolated rat islets. We have isolated two 20-mer peptides that bind to islets ex vivo. One of these peptides preferentially homes to the islets of Langerhans in a normal rat with clear differentiation between the endocrine and exocrine cells of the pancreas. Furthermore, this peptide does not target ß-cells in a type 2 diabetes animal model, suggesting that the peptide can discriminate between glucose-stimulated insulin secretion–functional and -dysfunctional ß-cells.

Abbreviations: GSIS, glucose-stimulated insulin secretion; HBSS, Hank’s balanced salt solution; RIP, rat islet peptide

The ß-cells of the islets of Langerhans in normal mammals adjust their secretion of insulin in response to changes in the levels of metabolic fuels and insulinotropic hormones. Loss of ß-cell function is central to the development of both major forms of diabetes. Type 1 diabetes occurs when pancreatic islet ß-cells are destroyed by the host immune system. Type 2 diabetes involves loss of key ß-cell functions such as glucose-stimulated insulin secretion (GSIS) and a gradual loss of ß-cell mass by nonautoimmune mechanisms. Intensive research efforts are currently focused on identifying pathways by which insulin secretion can be increased or ß-cell growth and survival can be enhanced. However, the therapeutic relevance of such discoveries for enhancing islet function or preserving ß-cell mass in pre-diabetic or diabetic states may be limited by the inability to deliver new therapeutic drugs, genes, or proteins directly to islet ß-cells. The current study attempts to address this issue by the application of phage-display technology for the identification of peptides that target specifically to ß-cells in pancreatic islets of living animals.

Specific delivery of molecular cargo to pancreatic islets has been a long-standing goal of diabetes researchers. Recombinant adenovirus and adeno-associated virus vectors have been used for efficient delivery of genes and, more recently, small interfering RNA constructs to primary cultures of pancreatic islets (1–4). However, these vectors have traditionally not been useful for delivery of genes to pancreatic islets of living animals because of very efficient clearance of systemically injected virus by the liver and the need to traverse vascular barriers in islets. Recently, some limited success in gene transfer (an average of 20% of cells in 70% of islets) has been reported in studies involving systemic infusion of adenovirus into mice in which the hepatic circulation (portal vein, hepatic artery, and bile duct) had been surgically clamped for a period of 30 min (5). The major surgical intervention required in this approach and the potential for immune responses to adenoviral vectors may limit its applicability for human studies. Another recent study presented an alternative strategy for islet targeting involving infusion of a cationic peptide transduction domain (PTD-5) fused to peptide inhibitor of IB kinase (IKK), resulting in improved islet function and viability upon subsequent isolation (6). Implementation of this strategy required infusion of the PTD-5/IKK inhibitor fusion peptide via the surgically resected bile duct, again seemingly limiting its broad applicability. Clearly, strategies for restoring ß-cell function and preserving islet mass in diabetes would be greatly aided by the ability to target genes, proteins, or small molecules in a more noninvasive and specific fashion than has been achieved to date. Furthermore, the ability to direct imaging agents specifically to ß-cells would facilitate diagnosis and monitoring of disease progression (7).

M13 phage-display technology is a powerful approach for isolating peptides that bind to cell surface receptors (8). In vivo phage panning has been successfully used to isolate peptides that mediate targeting to the vasculature beds of specific organs (9,10), including the pancreas (11). However, no accumulation of these selected peptides has been observed in the islets. Targeting to islets is made challenging by the fact that these cells in aggregate represent only 2% by weight of the entire pancreas (12). We have previously demonstrated that phage panning can be carried out on cells in culture to obtain peptides that mediate specific binding to the target cells while not binding to undesired cell types (8,13–17). The high discriminating power of the selected phage suggests that peptides could be identified that specifically bind to ß-cells within the pancreas. Furthermore, since intact cells are used as the bait for peptide binding, no prior information about ß-cell–specific cell surface biomarkers is required. Toward the eventual goal of delivering molecular cargo to ß-cells in a specific fashion in vivo, we have panned a phage-displayed peptide library on isolated rat islets and have isolated a 20–amino acid peptide that homes to the islets of Langerhans within living rats.

	RESEARCH DESIGN AND METHODS

TOP ABSTRACT RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

 
Cell lines and reagents.
A previously described random 20-mer peptide library, designated ON543.2, was used for the isolation of ß-cell–specific peptides (18). This library represents 10⁸ different peptide sequences displayed on the NH₂-terminus of the pIII protein of filamentous bacteriophage fd-tet. The INS-1–derived INS 832/13 cell line was maintained in culture as previously described (19). Female Sprague-Dawley rats were purchased from Harlan Industries (Indianapolis, IN). Male Zucker diabetic fatty (ZDF) rats were purchased from Charles River Laboratories (Wilmington, MA) and fed Purina Mills Formulab Diet 5008 (St. Louis, MO) to maintain their diabetic state (20,21). The experiments were performed with 12-week-old ZDF rats, at which time the animals were diabetic. All animal protocols were approved by the institutional animal care and research advisory committee at the University of Texas Southwestern Medical Center, Dallas, Texas.

Isolation of primary islets.
Primary islets were isolated from six female Sprague-Dawley rats weighing 225–250 g for each panning experiment according to standard protocols with minor modifications (22,23). Hank’s balanced salt solution (HBSS, pH 7.4; Invitrogen, Carlsbad, CA) supplemented with 1g/l of glucose and 200 mg/l BSA (Sigma-Aldrich, St. Louis, MO) was aerated with a 95% O₂ and 5% CO₂ gas mixture for 20 min on ice. The pancreas was perfused with 50 ml enzymatic digestion HBSS containing collagenase (112 units/ml; Sigma-Aldrich). Two pancreata at a time were treated by collagenase digestion at 37°C over a period of 21 min. During the first 5 min, the solution was aerated with 95% O₂ and 5% CO₂ gas, followed by continued incubation without the gas mixture for the next 4 min. The flask was vigorously shaken every 2 min for the remaining 12 min while being incubated. The digested pancreas was isolated by centrifugation, and discontinuous Ficoll (Amersham Biosciences, Piscataway, NJ) gradients in HBSS were used to separate islets. The samples were centrifuged at 500g for 20 min at 4°C. After collecting islets from all six rats, the islets were isolated by centrifugation at 200g and immediately used for panning.

Ex vivo phage library panning on primary rat islets.
The panning procedure was modified from previously published protocols (8,14) for use with freshly isolated islets. Preclearing of cell surface receptors was not necessary since islets were isolated in serum-free media. Islets in suspension were mixed with 3 x 10¹⁰ phage particles, 100 µmol/l chloroquine (Sigma-Aldrich), and 1 x protease inhibitor cocktail (Roche Diagnostics, Mannheim, Germany). Islets were incubated with phage for 1 h at 37°C with gentle shaking. The islets were washed twice by suspension in 1 ml HBSS, followed by one 1-ml wash with 0.1 N HCl-Glycine (pH 2.2). The cells were lysed by the addition of 1 ml hypotonic solution (30 mmol/l Tris-HCl, pH 8.0), followed by a single freeze-thaw cycle. The phage from the output fraction was amplified according to standard protocols for use in the next round of panning (24). Aliquots of the initial input and output samples were titered, and the output-to-input phage ratio based on colony-forming units was determined to monitor the progress of each round of library panning (24). To compare phage binding to cells, an output-over-input ratio was calculated as follows: output-to-input ratio = output titer of phage from lysed cells/input titer of total phage incubated with cells.

Sequence determination.
Random phage clones from titration plates were routinely sequenced after round 3 of the library panning to identify convergent peptide sequences as previously described (15). Convergent peptide-displaying phage clones were isolated for further characterization.

In vitro phage specificity panning.
Isolated phage clones selected from the library panning were characterized by panning on cell lines as previously described (14) using 2 x 10⁸ phage particles of each phage clone. Incubations were carried out for 1 h before the removal of unbound and surface-bound phages. Specificity panning on islets was performed in the same manner as the library panning with the exception that 2 x 10⁸ phage particles of a single-phage clone were placed on the purified islets from Sprague-Dawley rats. Colony-forming units were determined from bacterial titering of the output and input samples, and output-to-input ratios were calculated to determine phage binding.

In vivo phage delivery in Sprague-Dawley and ZDF rats.
Rats were anesthetized with pentobarbitol at 100 mg/kg and injected with 2 x 10⁸ phage particles via the jugular vein. After 2 h, the animals were perfused with 150 ml PBS via cannulation of the carotid artery. The abdominal cavity was opened to expose the liver to monitor blanching of this tissue during perfusion. Heart, lung, spleen, pancreas, skeletal muscle, kidney, and liver were harvested and fixed in Carson’s modified buffered formalin (Richard-Allan Scientific, Kalamazoo, MI) overnight. Paraffin processing, embedding, and sectioning were performed by standard procedures by the Molecular Pathology Core at the University of Texas Southwestern Medical Center.

Immunohistochemistry.
Paraffin-embedded tissue sections were deparaffinized using a Sakura Tissue-Tek DRS (Torrence, CA). Tissue samples were permeabilized with 0.5% Triton X-100 in PBS for 5 min at room temperature followed by blocking with 2% normal goat serum (Jackson ImmunoResearch Laboratories, West Grove, PA) in PBS⁺ (8.2 mmol/l Na₂PO4, 1.5 mmol/l KH₂PO4, 137 mmol/l NaCl, 2.7 mmol/l KCl, and 0.5 mmol/l CaCl₂, pH 7.4) containing 0.5% BSA for 40 min. Spleen samples were also blocked using FC-Block (1:200) (BD Pharmingen, San Diego, CA) to minimize non–antigen-specific binding. The samples were incubated overnight at 4°C with a 1:50 dilution of mouse anti-phage polyclonal antibody (15) or mouse monoclonal anti-insulin antibody (Sigma, St. Louis, MO) in PBS⁺/0.5% BSA. Excess antibody was washed off with PBS⁺ containing 0.5% BSA and a 1:24 dilution of fluorescein isothiocyanate–conjugated goat anti-mouse immunoglobulin antibody (Jackson ImmunoResearch Laboratories) was incubated with the tissues for 1 h at room temperature. Excess antibody was removed with serial washes with PBS, and a 1:5,000 dilution of Hoechst Dye #33342 (Molecular Probes, Eugene, OR) was used to stain nuclei. Tissue samples were covered with Vectashield (Vector Laboratories, Burlingame, CA). Tissue slides were evaluated and photographed via fluorescent microscopy on an Eclipse TE2000 fluorescent microscope (Nikon, Melville, NY) equipped with a CoolSNAP_fx camera (Roper Scientific, Tuscon, AZ). Images were captured using MetaVue v4.6r9 (Universal Imaging, Downington, PA) acquisition and analysis software.

	RESULTS

TOP ABSTRACT RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

 
Isolation of an islet-binding peptide from a peptide library.
To obtain peptides that recognize ß-cells in a biologically relevant system, freshly isolated pancreatic islets were used to pan a complex peptide phage library. This library contains 10⁸ different 20-mer peptides fused to the NH₂-terminus of the pIII coat protein of fd-tet bacteriophage. After six rounds of panning, a dramatic increase was observed in the output-to-input phage ratio, representing a 70-fold enrichment from the starting library (Fig. 1). Sequencing of 32 phage clones at round 6 of the panning revealed two major peptides. The first peptide, named rat islet peptide (RIP)-1, has the sequence LSGTPERSGQAVKVKLKAIP and was present in 15 of the 32 clones. The second peptide, RIP2, represented 25% of the phage clones and has the sequence GAWEAVRDRIAEWGSWGIPS. Sequencing of phage clones from earlier rounds of the panning process revealed that the RIP1 phage clone was present as early as round 4 of the panning protocol and was >20% of the phage pool at round 5. Surprisingly, the RIP2 sequence was not present until round 5 and then only as a single clone of the 28 sequenced. One other phage was present in duplicate in round 6, but because it represented <10% of the phage population and was not observed in earlier rounds of panning, this peptide was not retained for further analysis.

View larger version (11K): [in this window] [in a new window]   FIG. 1. The output-to-input ratio of bacteriophage increases over successive rounds of panning as binding phage clones are successively amplified and nonbinding phage clones are depleted. Binding of phage clones from round 6 is 70-fold greater than the complete library from round 1. Sequence results from round 6 indicate that RIP1 phage clone comprises 50% of the population and RIP2 comprises 25% of the population.

RIP1 and RIP2 peptides mediate binding to islets.
The binding of the RIP1 and RIP2 phage clones was tested on isolated islets, and the output-to-input phage ratio was used as a measure of phage binding to the islets. Both phage clones exhibit significant binding with 0.5% of the RIP1 phage and 7% of the RIP2 phage input being retained (Table 1). It is unexpected that the binding retention would be less for the RIP1 phage, which was the predominate clone in the phage selection. However, selection pressures other than cell binding can influence the isolation of phage clones, stressing the importance of assessing binding in vitro and in vivo of individual phage clones.

The RIP1 phage homes to the islets of Langerhans in living rats.
The true test of the relevance and potential applicability of our approach is to assess the ability of selected phage to target ß-cells in an animal. To test this, RIP1, RIP2, or a control phage containing a random peptide sequence were injected into the jugular vein of a rat. Phage was allowed to circulate for 2 h, after which the animal was killed and organs harvested. The presence of phage in islets and other tissues was then determined by immunohistochemistry using an anti-phage antibody. The results are shown in Fig. 2. In animals that received the RIP1 phage, phage immunostaining is clearly identifiable in the islets and the signal overlaps with insulin expression, suggesting that the phage is binding to the ß-cells. Diffuse, less intense staining is observed in the exocrine cells in the pancreas. Similar diffuse staining is seen throughout the pancreas of animals that have not received a phage injection or have been administered an irrelevant control phage, suggesting that this is background binding of antibody. However, we cannot rule out that the phage is also binding weakly to the nonendocrine cells of the pancreas. Similar but less dramatic preferential staining of the islets relative to the exocrine pancreas was obtained with the RIP2 peptide. Importantly, animals that were infused with the control phage containing a random peptide sequence exhibited no preferential phage immunolocalization in islets, indicating that the selected RIP1 and RIP2 peptides are mediating binding to the ß-cells and this staining pattern is not due to nonspecific uptake of the phage particles (online appendix [available at http://diabetes.diabetesjournals.org]).

View larger version (96K): [in this window] [in a new window]   FIG. 2. In vivo distribution of RIP1 and RIP2 phage in pancreata from Sprague-Dawley or ZDF rats. The phage was injected intravenously into the jugular vein of a rat and allowed to circulate for 2 h, after which the animal was killed and organs harvested. The presence of the phage was determined by immunohistochemistry using an anti-phage antibody. Aligned sections are shown staining with anti-insulin or anti-phage antibodies. All panels are at 100x magnification. Significant accumulation of RIP1 and RIP2 phage in the islets of the Sprague-Dawley rats is visible. No significant accumulation of RIP1 phage is seen within the islet of a ZDF rat.

View larger version (65K): [in this window] [in a new window]   FIG. 3. In vivo distribution of the RIP1 phage throughout a Sprague-Dawley rat. No significant phage accumulation is observed in muscle, heart, and lung. Nonspecific clearance of phage can be seen in liver, spleen, and kidneys. All panels are at 100x magnification.

	DISCUSSION

TOP ABSTRACT RESEARCH DESIGN AND METHODS RESULTS DISCUSSION REFERENCES

 
The ability to target genes and therapeutics specifically to ß-cells would facilitate diabetes treatment. Furthermore, determination of ß-cell mass and function in vivo has been hampered by the inability to direct imaging agents to ß-cells within the pancreas. Typically, cell-specific delivery is achieved by attaching the desired biomolecule to a ligand for a well-characterized cell surface molecule that is preferentially expressed in the targeted cell type. Using antibodies as the homing agent, this approach has been used for tumor-specific delivery of chemotherapeutics (27,28), and several immunotherapies are currently in the clinic (29). However, little is known about the cell surface profile of ß-cells, and currently, the IC2 antibody is the only ligand used for delivery to ß-cells in animals (30,31).

To circumvent the need for a defined biomarker, we used biopanning to isolate peptides that bind to islets of Langerhans from normal Sprague-Dawley rats. After six rounds of reiterative panning, the output-to-input phage ratio increased 70-fold. From a phage-displayed peptide library representing 10⁸ different members, we isolated two 20–amino acid peptides, RIP1 and RIP2, that bind to islets ex vivo as determined by phage retention. It is important to note that little similarity is observed between the RIP1 and RIP2 peptide sequences, suggesting that they are most likely binding to different cellular receptors or different binding pockets within the same receptor. Furthermore, neither of these peptides show significant sequence similarity to previously isolated peptides that home to the pancreas vasculature (11). A BLAST analysis for short peptides of similar sequence revealed no significant homologies to known proteins in the NCBI database (25).

The major goal of this study was to identify peptides that mediate binding to ß-cells within a living animal. Realization of this goal requires that the identified peptides have a significantly higher affinity for ß-cells than for other cell types, the phage clones can escape the vasculature to reach the appropriate cells, and the peptide is stable in vivo. To address this, the isolated RIP1 and RIP2 phage clones were injected into normal Sprague-Dawley rats, followed by harvesting of tissue and immunohistochemical analysis with anti-phage antibodies to determine the phage localization. The RIP1 phage preferentially homes to the islets of Langerhans in a normal rat with differentiation between the endocrine and exocrine cells of the pancreas. The immunohistochemical signal is observed throughout the islet and colocalizes with staining obtained with anti-insulin antibodies, indicating that the phage clone is binding to the ß-cells within the islets. The RIP1 phage is not enriched in other tissues, although a nonspecific signal is observed in liver and kidney that is equal in intensity to that observed following injection of a control phage containing a random peptide sequence. We suspect that this signal is due to nonspecific clearance of the phage, but at this time, we cannot rule out that the peptide has some affinity for these cells as well. The RIP2 phage also accumulates in the islets, but the preferential localization to endocrine cells is less pronounced than observed with the RIP1 phage, even though the RIP2 displayed higher phage retention on islets in vitro. Furthermore, this phage showed significant accumulation in tissues and organs, indicating that this peptide binds nonspecifically to different cell types.

Because the RIP1 phage was selected on islets from healthy Sprague-Dawley rats, we sought to determine whether this phage clone could also target to ß-cells in ZDF rats at 12 weeks of age, at which time the animals are severely diabetic and exhibit defective GSIS. We found that the RIP1 phage does not target ß-cells in diabetic ZDF rats. This suggests that this peptide is recognizing a cell surface feature on normal, fully functional ß-cells that is lost or obscured during disease progression. This cell surface feature might be related to the loss of GSIS, or alternatively, may be influenced by the increased infiltration of fibrotic tissue or the increased rate of cell death that occurs in ZDF islets in concert with progression to diabetes (32,33). Further studies will be required to determine whether RIP1 phage are able to target ZDF islets before onset of diabetes and conversely whether peptides can be identified that bind specifically to islets in diabetic animals.

In summary, we have isolated a peptide that is able to home to normal ß-cells in the islets of Langerhans without prior knowledge of a ß-cell biomarker. We anticipate that this peptide will be of utility for ß-cell–specific delivery of molecular cargo, possibly including plasmids that contain specific therapeutic/protective genes, bioactive peptides or proteins, small molecules, or imaging agents. Use of the RIP1 peptide for these purposes will require demonstration of the ability of the isolated peptide, removed from the context of phages, to target islets in a manner similar to what has been observed for the phage clone. The peptide will then be utilized to deliver active biomolecules to the target cells. While these are significant hurdles, the current study provides promise for the use of selected peptides for islet-specific targeting applications in the near future.

	ACKNOWLEDGMENTS

 
This work was supported by a Program Project Grant from the National Institutes of Health (5PO1 DK-05839805).

We thank Kimberly Jones-Ross for helpful experimental suggestions for islet isolation and Shuyuan Chen for technical expertise in establishing the in vivo delivery experiments. We also thank James A. Richardson, John M. Shelton, and the Molecular Pathology Core for their contribution to the processing of tissue samples and slide preparation. Ya-Ching Chang and Chun Man Lee contributed technical assistance.

	FOOTNOTES

 
Additional information for this article can be found in an online appendix at http://diabetes.diabetesjournals.org.

Received for publication January 24, 2005 and accepted in revised form April 11, 2005

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