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The Journal of Neuroscience, September 15, 1999, 19(18):7732-7741
Insulin Prohormone Processing, Distribution, and Relation to Metabolism in Aplysia californica
Philip D. Floyd1, Lingjun Li1, Stanislav S. Rubakhin1, Jonathan V. Sweedler1, Charles C. Horn2, Irving Kupfermann2, Vera Y. Alexeeva3, Timothy A. Ellis3, Nikolai C. Dembrow3, Klaudiusz R. Weiss3, and Ferdinand S. Vilim3 1 Department of Chemistry and the Beckman Institute, University of Illinois, Urbana, Illinois 61801, 2 Center for Neurobiology and Behavior, Columbia University, New York, New York 10032, and 3 Department of Physiology and Biophysics, Mount Sinai School of Medicine, New York, New York 10029
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
The first Aplysia californica insulin gene is characterized and its proteolytic processing from prohormone to final peptides elucidated using a combination of biochemical and mass spectrometric methods. Aplysia insulin (AI) is one of the largest insulins found, with a molecular weight of 9146 Da, and an extended A chain compared with other invertebrate and vertebrate insulins. The AI prohormone produces a series of C peptides and also a unique N-terminally acetylated D peptide. AI-producing cells are restricted to the central region of the cerebral ganglia mostly within the F and C clusters, and AI is transported to neurohemal release sites located on the upper labial and anterior tentacular nerves. The expression of AI mRNA decreases when the animal is deprived of food, and injections of AI reduce hemolymph glucose levels, suggesting that the function of insulin-regulating metabolism has been conserved.
Key words: insulin; neuropeptide; Aplysia californica; cerebral ganglion; hunger/satiation; glucose
INTRODUCTION
Insulin is one of the most extensively studied protein hormones found in a diverse range of species ranging from humans (Banting and Best, 1922
) to unicellular organisms and plants (Collier et al., 1987
Immunocytochemical evidence indicates that these insulin-like peptides are present in the CNS of Aplysia californica (Van Minnen and Schallig, 1990
Surprisingly, after cloning the insulin receptor and these functional studies, no insulin peptide or gene has been found in Aplysia, although several insulin-like peptides have been isolated in other mollusks (Smit et al., 1988
MATERIALS AND METHODS
Animals. Aplysia californica weighing 10-200 gm were obtained from Aplysia Research Facility (Miami, FL), whereas those weighing 200-350 gm were purchased from either Pacific Biomarine (Venice, CA) or Marinus, Inc. (Long Beach, CA), and larger animals (up to 2 kg) were collected from McAbee Beach in Monterey, CA. Animals were maintained in artificial seawater (Instant Ocean; Aquarium Systems, Mentor, OH) at 14°C.
Cellular sample preparation. Ganglia and cellular clusters with intact connectives and commissures were removed after injection of 390 mM MgCl2 equal to one-half of each animal's body weight. In some cases, a moderate protease treatment (e.g., 1% protease type IX for 30-60 min at 34°C) was used to soften the connective tissues before desheathing.
Matrix-assisted laser desorption-ionization mass spectrometry. Mass spectra were obtained using two mass spectrometers, namely a Voyager Elite and a Voyager DE STR equipped with delayed ion extraction (PE Biosystems, Framingham, MA). A pulsed nitrogen laser (337 nm) was used as the desorption/ionization source, and positive-ion mass spectra were acquired using both linear and reflectron mode. Each representative mass spectrum shown is the unsmoothed average of 64-128 laser pulses. Mass calibration was performed externally using either bovine insulin (Sigma, St. Louis, MO) or a previously calibrated spectrum obtained from Aplysia bag cells. The averaged mass assignment error is 190 ppm for linear mode, which is typical for the cellular peptide assay using external calibration (Li et al., 1998
Microbore RP-HPLC of homogenates. Cerebral F and C clusters from 23 animals were pooled for microbore RP-HPLC separation. The clusters were collected on dry ice and subsequently stored at
80°C in ~200 µl of acidified acetone (1:40:6, HCl:acetone:H2O) as described previously (Newcomb and Scheller, 1990
In all cases, the samples were collected by a fraction collector (FC 203B; Gilson, Middletown, WI), and each fraction was screened by MALDI-MS; 0.25 µl of each liquid chromatography (LC) fraction was deposited onto a MALDI-MS sample plate followed by the same volume of 10 mg/ml
-cyano-4-hydroxy-cinnamic acid (dissolved in 6:3:1 acetonitrile:water:3% TFA) (Aldrich, Milwaukee, WI) or aqueous dihydroxybenzoic acid (ICN Biochemicals, Costa Mesa, CA) (10 mg/ml) matrix solution. Unless otherwise specified, all solvents were purchased from Fisher Scientific and were reagent quality or better.
Cloning. Standard molecular techniques (Sambrook et al., 1989
phage library (Stratagene, La Jolla, CA), was used both as a template for PCR and for conventional hybridization screening. Semi-nested degenerate rapid amplification of cDNA ends (RACE) was performed using two vector primers and an antisense degenerate primer designed to a subset of the peptide sequence (NVNDKLRGIL = ard ati cci cki ary ttr tcr tti acr tt). PCR was performed in two stages on a robocycler gradient 40 thermal cycler (Stratagene) using taq DNA polymerase and dNTPs from Perkin-Elmer (Norwalk, CT). Both stages were cycled 25 times with 30 sec at 95°C, 1 min at the annealing temperature, and 2 min at 72°C. Three separate annealing temperatures (50, 54, and 58°C) were run in parallel, and a set without the degenerate primer was used as a control. The reactions were hot started and not allowed to cool to <72°C between the stages. In the first stage, 10 µl reactions containing 0.1 µM vector primer (ACC ATG ATT ACG CCA AG), 0.1 µM degenerate primer, 100 µM dNTPs, and 0.1 µl of library were hot started with 0.1 U of taq in 0.5 µl of reaction buffer. In the second stage, 50 µl of prewarmed (72°C) reaction mix containing 1 µM nested vector primer (GAA ATT AAC CCT CAC TAA AGG), 1 µM degenerate primer, and 100 µM dNTPs were added to each tube, then hot started again with 1 U of taq. The results of the PCR were assessed using agarose gel electrophoresis and the highest temperature reactions showing significantly more product than the matched degenerate primerless control were polyethylene glycol 8000-precipitated and TA-cloned (Invitrogen, Carlsbad, CA). Insert-bearing clones were identified using colony PCR then cycle-sequenced by dye termination (Perkin-Elmer, Norwalk, CT). Inserts from promising degenerate clones were isolated and labeled using 32P-dCTP and random primers (New England Biolabs, Beverly, MA). These probes were then used to screen a library to identify full-length clones. Three clones were sequenced to generate a consensus. Sequence alignments were generated using Geneworks version 2.1, and consensus contigs were assembled manually.
Northerns. Like ganglia were dissected and pooled from five animals anesthetized with 50% volume of isotonic MgCl2. The RNA was isolated by the acid phenol method (Chomczynski and Sacchi, 1987
Antibodies. The antigen was prepared by coupling Aplysia insulin C
(DTENVNDKLRGILLN) to BSA (SIGMA A0281) using either 1-ethyl-3-(dimethylaminopropyl)carbodiimide (EDC) (SIGMA E7750) or paraformaldehyde/glutaraldehyde (Pf/G; EM Sciences, Fort Washington PA). The coupling was performed in a 0.5 ml volume of 50 mM NaH2PO4, pH 7.2, containing 5 mg of BSA, 1 mg of peptide, and either 10 mg of EDC or 1% paraformaldehyde and 0.1% glutaraldehyde. The mixture was allowed to react overnight at 4°C and then the coupled antigen was purified from the reaction using a Microcon-30 (spinning at 13,800 × g for 30 min at 4°C to concentrate). After washing the retentate four times with 0.4 ml of 50 mM NaH2PO4, pH 7.2, it was resuspended in 0.25 ml of the same buffer and transferred to a new tube.
Four male Sprague Dawley rats (Teconic; 250-300 gm) were immunized by intraperitoneal injection with 12.5 µl (~250 µg) antigen in an emulsion of 0.5 ml PBS and 0.5 ml of Freund's complete adjuvant. At 21 and 42 d after initial injection, the rats were boosted by intraperitoneal injection with 6.65 µl (~125 µg) antigen in an emulsion of 0.5 ml PBS and 0.5 ml of Freund's incomplete adjuvant. The animals were sacrificed by decapitation at 49 d after initial injection, and the blood was harvested and processed for serum. Sera were aliquoted, frozen, and lyophilized, or stored at 4°C with EDTA (25 mM final) and thimerosal (0.1% final) added as stabilizers.
Immunocytochemistry. Immunocytochemistry was performed as previously described (Vilim et al., 1996
Food deprivation experiments. Twenty animals that had been starved for 0, 1, 2, and 3 weeks were obtained from the Aplysia Research Facility (Miami, FL). They were all 100-110 gm and were the same age when the experiment started. The experiment was designed such that the animals would all arrive on the same day. The animals were shipped on ice and processed on arrival without letting the animals warm. The ganglia from each animal were removed, combined and processed for RNA as described above. Northern analysis proceeded as above, and densitometric analysis of the scanned autoradiographs was performed using NIH Image (version 1.55). Statistical significance of differences between control and starved animals was determined with Student's t test.
Hemolymph glucose experiments. Aplysia insulin (AI) was isolated from 100 Aplysia cerebral ganglia and subjected to multiple RP-HPLC separations until a peak with 80% purity (by MALDI-MS) at 9146 Da was obtained. The effect of the authentic AI on hemolymph glucose level was measured. Animals (129-200 gm) were tested after 3 d of food deprivation to assure that the crop was empty of food during the experiment, and were injected on the test day with 1 ml of artificial sea water (ASW) (n = 7) and AI (~100 pmol of native AI in 1 ml of ASW; n = 6) into the hemocoel with a syringe needle (26 gauge). We also tested synthetic acetyl-TGR peptide (~1.07 mM per animal, 1 ml; n = 4), which is the first three amino acids of the insulin "D-peptide", and was of interest because no other known insulin prohormone contains this peptide. Hemolymph glucose was measured enzymatically using the glucose oxidase method (Trinder, 1969
RESULTS
MALDI-MS of single top-layer cerebral F cluster (CFt) neurons identified a peak with a mass of 1714 Da that did not correspond to any known neuropeptide (Rubakhin et al., 1999
F and C clusters were pooled from 23 animals, homogenized, lyophilized, and subjected to three separate rounds of HPLC separations using MALDI-MS to track the 1714 Da peak. The output of the final separation (Fig. 1, inset) was a peptide with sufficient amount and purity to be sequenced. The N-terminal sequencing analysis on this sample via Edman degradation revealed a sequence of: XTXNVNDKLRGILLN (with X indicating unassignable residue) that was used for subsequent PCR analysis.
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Figure 1. Representative mass spectrum of a top layer neuron from the F cluster in the cerebral ganglion. Peaks generally correspond to [M+H]+, where M is the molecular weight of each peptide. Aplysia insulin (AI), and its shortened form AI', C
Semi-nested degenerate PCR yielded a single clone which, upstream of the degenerate primer, encoded the predicted upstream amino acid sequence. The correct clones were used to screen a library and isolate three clones. The longest insert was ~4.5 kb. The mRNA shown in Figure 2 consists of a 468 bp open reading frame that codes for a 156 amino acid precursor containing a single copy of the 1714 Da peptide (underlined in figure). Northern analysis (Fig. 3) indicates that the mRNA is ~4.5 kb in length, suggesting that the clones isolated from the library were near full length. Sequencing of the 5' 1 kb of these three clones yielded consensus sequence for the entire coding region. The 3' end of the mRNA has not been sequenced, but the 190 bp of 3' untranslated region sequenced contains multiple stop codons in all three frames, indicating that the remaining 3.2 kb of 3' sequence is also untranslated region. The predicted amino acid sequence does, in fact, show considerable homology to the insulin family of prohormones and represents the first of its kind to be reported in Aplysia.
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Figure 2. cDNA and predicted protein sequence of the Aplysia insulin prohormone (GenBank accession number AF160192). The nucleotide sequence of the strand corresponding to the mRNA is shown with 5' and 3' untranslated in lowercase letters and the coding region in uppercase letters. Nucleotide sequence in the coding region is grouped by codons with the coded amino acid shown below. Numbering of amino acids and nucleotides is shown at the end of each line with nucleotide numbering negative before the coding sequence and positive after the 5' untranslated region. Predicted proteolytic processing sites are shown in bold, and the predicted signal sequence proteolytic processing site is shown with an asterisk. The sequence of the biochemically purified and sequenced peptide is underlined.
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Figure 3. Northern analysis of AI mRNA. A, Methylene blue staining of total RNA isolated from the different ganglia of Aplysia. The equal density of the rRNA band (which runs as a single 18 sec band) demonstrates equal loading of RNA in all lanes. The size and positions of the RNA markers are shown to the left. M, RNA marker lane; B, buccal ganglia; C, cerebral ganglia; L, pleural ganglia; E, pedal ganglia; A, abdominal ganglia. B, Hybridization of the total RNA with probe to the insulin mRNA. The hybridizing RNA is present only in cerebral ganglion total RNA and shows a principal band at ~4.5 kb. Lower molecular weight (<1 kb) hybridizing RNA in the cerebral ganglia is most likely the result of degradation products of the full-length mRNA.
Several criteria confirm that the isolated clone represents the precursor to the peptide originally isolated and sequenced from F cluster neurons. First, the amino acid sequence of the 1714 Da peptide is found on the precursor (Fig. 2, underlined sequence) and it is flanked by dibasic processing sites, indicating that it can be proteolytically cleaved from the precursor. Second, the Northern analysis (Fig. 3) shows that the precursor mRNA is present exclusively in the cerebral ganglia, where the F cluster is located. Third, immunocytochemistry directed against the 1714 Da peptide sequence stains neurons in the F cluster of the cerebral ganglia and the UL and AT nerves (Fig. 4). Furthermore, the immunostained neurons in the F cluster have a similar morphology and distribution as the CFt class of neurons, which were the basis for the purification of the peptide (Rubakhin et al., 1999
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Figure 4. C
The amino acid sequence of the precursor predicts several processing sites of the prohormone convertase/furin family of endoproteases (Fig. 2, shown in bold). These dibasic or RXXR sites are cleaved C-terminal to the last basic residue, then carboxypeptidase E removes the C-terminal basic residues. If the next C-terminal residue is a glycine, peptidyl-glycine
When combined with the prohormone sequence, MALDI-MS is a powerful tool to confirm expected cleavage and determine unexpected processing steps. Because the cells synthesizing AI are easily isolated from the cerebral cluster (Rubakhin et al., 1999
Consistent with the targeting of the precursors to the release pathway, the precursor has a hydrophobic signal peptide. Using SignalP version 1.1 signal sequence predictor (Nielsen et al., 1997
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Figure 5. A, MALDI-MS of a C cluster homogenate before and after DTT treatment, illustrating cleavage of insulin disulfide bonds resulting in the appearance of A (4057 Da) and B (5093 Da) chains. B, Mass spectra of single F cluster neuron (top trace) and AT nerve (bottom trace) showing processing of C
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Table 1. Peptides from the AI prohormone The A and B chains together add to 9151 Da. When examining a single CFt cell (Fig. 1) that was not incubated in DTT, a strong peak is observed close to this mass that disappears with DTT treatment. When deducing the structure of the A and B chains, one notices the presence of four possible Cys-Cys bonds. Each Cys-Cys bond results in the loss of 2 Da. Single cells and purified LC fractions containing AI were examined with high mass accuracy using reflectron mode. The observed mass is 9146.5 (
= ±0.9; n = 10), suggesting the presence of three disulfide bonds, and confirming the presence of between two and four disulfide bonds.
Interestingly, a second peak at 8626 Da also disappears in the presence of DTT (Fig. 1). This appears to be a modified form of AI (AI'), consisting of a truncated B chain that involves a cleavage at the single basic residue K[73] and results in the removal of C-terminal residues KYMV from the B chain of AI, with the shortened form of the B chain (assigned as B-chain' with molecular weight at 4572 Da) observed after treatment with DTT. Besides observing the AI and AI' (removal of KYMV), MALDI-MS also detects the presence of two additional peaks that correspond to the removal of C-terminal residues V and M, respectively. This observation is likely caused by the MALDI-MS in-source decay process (Brown and Lennon, 1995
The AI prohormone contains two peptides located between the A and B chains. These are designated as C
and C
Examining the prohormone sequence shown in Figure 2, there is an additional peptide after the A chain, specifically T[141]-S[156]. Such an extra peptide is unique to AI compared with other known insulin prohormones, although insulin growth factors (IGFs) contain a D domain that is not proteolytically cleaved from the rest of the prohormone. We observe this mass in LC fractions and single cells, as well as a peak exactly 42 Da higher, indicating putative acetylation of the peptide. We also observe an intense peak corresponding to cleavage at the R[143], leaving the peptide S[144]-S[156] without the +42 Da peak, indicating the acetylation is in the N-terminal 3 amino acids, and most likely on the N-terminal threonine. The appropriate LC fractions have been sequenced, which confirms our assignments of both the D peptide and shortened form in the mass spectra. Because of limitations of MALDI-MS in observing the <300 Da range because of the interference from the MALDI-MS matrix, we have been unsuccessful in observing the putative acetyl-TGR peptide. In addition, it is possible that this peptide is present in the shortened forms T-amide, acetyl-T-amide, or acetyl-TG. These are the only masses, besides the signal sequence, not directly confirmed with mass spectrometry.
Both the putative acetylated and native peptides are observed in LC fractions and in single cells. An important question is whether both the acetyl and non-acetyl peptides are present in cells. The 0.1% TFA used in the first stage of the LC separations has been reported to partially remove acetyl groups from peptides (Gheorghe et al., 1997
The distribution of AI precursor was examined using antibodies to the C
To investigate the effects of food deprivation on AI mRNA expression, a group of Aplysia of similar size and age were starved for 1, 2, and 3 weeks. The mRNA levels for AI, actin, cerebral peptide 2 (CP2) and myomodulin (MM) were measured, with the results shown in Figure 6. As indicated, AI precursor mRNA levels drop significantly (p < 0.001) after 2 and 3 weeks of food deprivation. Actin mRNA levels also dropped significantly (p < 0.05) after 2 and 3 weeks of food deprivation. Although CP2 mRNA levels showed a decreasing trend, and MM mRNA levels showed an increasing trend with longer food deprivation, these results were not statistically significant. Thus, the decline in AI mRNA with food deprivation cannot be attributed to some generalized decline in mRNA levels. It should be noted that although CP2, MM, and AI mRNA are found exclusively in neurons, actin mRNA is present in the ganglia sheath as well as the neurons. Thus, the decrement of actin mRNA resulting from prolonged food deprivation may represent the downregulation of the synthesis of contractile machinery in the sheath.
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Figure 6. Effect of food deprivation on insulin, cerebral peptide 2 (CP2), myomodulin, and actin mRNA levels. Error bars indicate mean ± SEM of mRNA levels measured from five animals after 0, 1, 2, and 3 weeks of food deprivation. Asterisk denotes statistically significant differences as compared with non-food-deprived controls. CP2 and myomodulin mRNA levels did not change significantly, whereas insulin (p < 0.001) and actin (p < 0.05) mRNA showed significant decreases after 2 and 3 weeks of starvation.
To determine if Aplysia insulin may be involved in the regulation of hemolymph glucose, AI was injected into food-deprived animals. Injection of AI significantly decreased hemolymph glucose at 1.5 and 3 hr compared with control injection of ASW (Fig. 7; F(4,28) = 4.73; p < 0.005; p values < 0.05, Tukey's HSD comparisons). The Aplysia insulin prohormone fragment, acetyl D-TGR peptide, had no effect on hemolymph glucose levels compared with control injection of ASW. There were no obvious behavioral effects in any of the injected animals, including no egg laying.
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Figure 7. Effect of AI and the acetyl D-TGR peptide on hemolymph glucose in food-deprived Aplysia. At 1.5 and 3 hr after injection of AI hemolymph, glucose was significantly decreased compared with control injection of ASW. The acetyl D-TGR peptide had no effect on hemolymph glucose. Values are means ± SEM. *p < 0.05 versus ASW control, Tukey's HSD test.
DISCUSSION
The AI prohormone undergoes complex processing to yield a series of peptides including AI, several C peptides, and a unique D peptide. Figure 8 summarizes the processing scheme and indicates whether each resulting peptide was observed with MALDI-MS, biochemically characterized, or merely predicted. As can be seen, for all major steps, the peptides have been confirmed with multiple techniques. Figure 9 compares a few of the reported insulin prohormones from locust to human and illustrates the similarities.
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Figure 8. Summary of insulin processing based on single-cell MALDI-MS and biochemical characterization. Inset shows AI with the A and B chains connected with putative disulfide bonds.
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Figure 9. Comparison of the AI prohormone structure to those of Lymnaea, human, and locust. As the AI precursor exhibits a D peptide region, it contains characteristics of both insulin and insulin growth factors in addition to being the largest molecular weight insulin reported to date.
Table 2 compares the amino acid sequence of AI to those of Lymnaea molluscan insulin-related peptides (MIPs) and human insulin. The A chains of both MIPs and AI appear to be terminally blocked (N-terminal pGlu). Comparison of amino acid sequence of the B chain and A chain shows that AI is homologous to MIPs with average sequence identity ~45%, ranging from 40 to 62%. Human insulin and AI do not share significant amino acid sequence similarity. However, all the residues that are important for the maintenance of the basic insulin core structure are conserved. As illustrated in Table 2, the spacing between cysteine residues are the same for all insulin species, suggesting that the characteristic disulfide bridges in the insulin molecules have been conserved. In addition, the hydrophobic core residues responsible for globular insulin structure are either conserved as identical residues or are replaced by equivalent hydrophobic residues.
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Table 2. Amino acid sequence comparison of insulins Aplysia insulin is the largest reported insulin peptide (~9146 Da) with greatly extended A and B chains. It is substantially larger than the MIPs isolated from Lymnaea stagnalis (Smit et al., 1998
The presence of a C peptide is conserved across all insulin prohormones, however a definitive function for the C peptide has yet to be determined. Ido et al. (1997)
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Table 3. Comparison of amino acid sequence of insulin C peptides The AI C
Perhaps the most interesting aspect of this AI prohormone is the D peptide. In other insulins, the prohormone ends with the A chain. For the AI prohormone, a unique peptide is encoded and its expression confirmed with both MALDI-MS and biochemical isolation and sequencing. Interestingly, the D peptide is acetylated, and we observe (again both by MALDI-MS of a single cell and biochemically) a shortened form consisting of the removal of the ac-TGR. The only members of the insulin superfamily that have extra peptides are the locust insulin (Lagueux et al., 1990
Insulin in many species is associated with food intake and metabolism (Woods, 1995
Several studies have demonstrated the biological effects of insulin on Aplysia. The exposure of bag cells to mammalian insulin was shown to induce autophosphorylation of the bag cell receptors and elevate voltage-dependent Ca2+ and K+ currents, which regulates the excitability of these neurons (Jonas et al., 1996
Although the most well known function of insulin in vertebrates is related to glucose metabolism, recent research suggests that insulin plays important roles in learning and memory (Wickelgren, 1998
FOOTNOTES Received May 10, 1999; revised June 28, 1999; accepted July 2, 1999.
This work was supported by the National Institutes of Health Grants NS31609, MH50235, K05MH01427, MH11586, and MH35564, and National Science Foundation Grant CHE 9622663. We gratefully acknowledge the generous gift of Aplysia cDNA library from Dr. Gregg Nagle. We also thank Tatiana Moroz for assistance in cell isolation and Midwest Analytical, Inc. for peptide sequencing. Aplysia californica were partially provided by the National Resource for Aplysia at the University of Miami under National Institutes of Health National Center for Research Resources Grant RR10294.
Correspondence should be addressed to J. V. Sweedler, 600 South Mathews Avenue, University of Illinois, Urbana, IL 61801.
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