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Lens Proteomics: Analysis of Rat Crystallin Sequences and Two-Dimensional Electrophoresis Map

¹ From the Departments of Oral Molecular Biology and ⁴ Ophthalmology, Schools of Dentistry and Medicine, Oregon Health and Science University, Portland, Oregon; and the ² Department of Animal Sciences, Oregon State University, Corvallis, Oregon.

	Abstract

Top Abstract Introduction Methods Results Discussion References

 
PURPOSE. To determine the sequence of four rat ß-crystallins, confirm the sequences by mass spectrometry, and produce a two-dimensional electrophoresis (2-DE) map of soluble crystallins in young rat lens.

METHODS. New or additional sequences were determined for ßB1, ßB3, ßA3, and ßA4-crystallin cDNAs from Sprague-Dawley rats, and the deduced protein sequences confirmed by mass spectrometry. The identity and relative abundance of each crystallin was then determined by 2-DE of soluble protein from whole lenses of 12-day-old rats, image analysis, and tandem mass spectrometry (MS/MS) spectra of peptides from in-gel digests.

RESULTS. The previously unreported sequence of rat ßA4 cDNA encoded a 195-amino-acid protein. Additional cDNA sequencing provided the previously unknown N-terminal sequence of rat ßA3, found two differences from the previous amino acid sequences of both rat ßB1 and ßB3, and detected a polymorphism at residue 54 in rat ßB3. These new sequences were then confirmed by whole protein masses and MS/MS spectra of proteolytic digests. 2-DE analysis provided a more detailed map of rat crystallins than previously available and allowed the composition of crystallins in young rat lens to be compared with that in young human lens.

CONCLUSIONS. This report provides baseline data that will facilitate the analysis of posttranslational modifications in rat crystallins during cataract. Detection of a polymorphism in the sequence of rat ßB3 suggests that crystallins in humans could also exhibit polymorphisms. The unusual abundance of rat ßB3 and low abundance of ßB2 may account for the increased susceptibility of rat crystallins to insolubilization during aging and cataract.

	Introduction

Top Abstract Introduction Methods Results Discussion References

 
Rodents remain the most common experimental animals used to study the mechanisms of cataract formation. This report describing the composition and sequences of rat crystallins and the accompanying report describing the composition and age-related changes in mouse crystallins¹ provide baseline information to assist in the detection of cataract-specific modifications in lens proteins.

Several experimental treatments used to induce cataracts in rats include streptozotocin-induced diabetes, galactose feeding, ionizing radiation, inhibition of cholesterol synthesis, steroid treatment, overdose of selenite, and culture with oxidants or calcium ionophore.^{2 3 4 5 6 7 8 9} In most of these models, covalent modification of crystallins, followed by phase separation of lens cytosol and formation of water-insoluble aggregates, may play important roles in opacification. Some of the modifications detected in rat crystallins that could contribute to insolubilization are mixed disulfide formation; glycation; cross-linking by UV, transglutaminase, or disulfides; phosphorylation; deamidation; and proteolysis.^{10 11 12 13 14 15 16}

Two-dimensional electrophoresis (2-DE) and mass spectrometric analysis, tools used in the emerging field of proteomics,¹⁷ hold great promise for determining which crystallin modifications lead to cataract. 2-DE is capable of simultaneously resolving complex mixtures of modified crystallins. These resolved crystallins can then be quantified by image analysis, and posttranslational modifications on excised spots can be determined by mass spectrometry (MS). To perform these studies, it is essential that the complete sequences of crystallins be known so that experimental and calculated masses may be compared. Furthermore, standardized 2-DE maps are required for reference to determine which species represent modified crystallins and which are cataract specific. Therefore, the purpose of this study was to determine the cDNA sequences of several rat ß-crystallins that were either unknown or were inconsistent with preliminary mass spectrometric data, to proofread the newly deduced sequences of ß-crystallins by measuring masses of whole crystallin subunits and peptide digests, and to produce a standardized 2-DE map of crystallins for young rat lens.

	Methods

Top Abstract Introduction Methods Results Discussion References

 
Isolation of RNA and Protein from Rat Lens
Lenses for RNA isolation were obtained from 12- to 28-day-old Sprague-Dawley rats (BK International, Fremont, CA). Treatment of animals conformed to the ARVO Statement for the Use of Animals in Ophthalmic and Vision Research. Lens mRNA and total RNA was isolated from dissected tissue, by means of a kit (Fast Track; (Invitrogen Life Technologies, Carlsbad, CA) and RNA extraction reagent (TRIzol; Invitrogen Life Technologies), respectively. Soluble crystallins were isolated from 12-day-old rats by homogenization, using a ratio of 20 lenses/mL of buffer containing 20 mM phosphate, 1 mM EGTA (pH 7.0), and one freshly added tablet of protease inhibitor/10 mL buffer (Complete Mini Protease Inhibitor Cocktail; Roche Molecular Biochemicals, Indianapolis, IN). The water-soluble and -insoluble fractions were separated by centrifugation at 20,000g for 30 minutes at 4°C. Protein content was measured using the bicinchoninic acid (BCA) assay and bovine serum albumin standard (Pierce, Rockford, IL).

Sequencing of Rat ßA4, ßA3, ßB1, and ßB3 cDNAs
After reverse transcription, the cDNA for rat ßA4 was amplified by PCR, using both the 3' and 5' rapid amplification of cDNA ends (RACE) systems (Invitrogen Life Technologies), as previously described.¹⁸ Gene specific RACE PCR primer sequences were designed using the previously published sequence of bovine ßA4 (GenBank accession no. M60328; GenBank is provided in the public domain by the National Center for Biotechnology, Bethesda, MD, and is available at http://www.ncbi.nlm.nih.gov/genbank) so that the sequence of the 5' and 3'RACE PCR products overlapped. PCR products were then cloned and plasmid DNA isolated as previously described.^{18 19}

To amplify the unknown 5' end of rat ßA3 cDNA, the same procedure described for the 5'RACE of rat ßA4 cDNA was used, except a gene-specific primer targeted to nucleotides 134-153 and a nested primer targeted to nucleotides 43-62 of the published 3' sequence of rat ßA3 were used (GenBank accession no. X15143).

Preliminary mass spectrometric analysis of rat ßB3 and ßB1 indicated that the calculated and experimentally measured masses did not match. Therefore, cDNAs coding for each protein were sequenced. Standard PCR was performed with primers corresponding to nucleotides 3-22 and 692-709 of ßB3 (GenBank accession no. X05899) or with primers corresponding to nucleotides 76-97 (GenBank accession no. M13527) and nucleotides 603-624 of ßB1 (GenBank accession no. X05900). The PCR product of rat ßB1 cDNA was cloned (Original TA cloning kit; Invitrogen Life Technologies). The PCR product of rat ßB3 cDNA was purified (QIAquick PCR Purification kit, Qiagen, Valencia, CA) and directly sequenced, using the same primers as were used for the original PCR. All DNA sequencing was performed by the Oregon Health and Science University Molecular Microbiology and Immunology (OHSU-MMI) Research Core Facility (http://www.ohsu.edu/core).

Isolation of ß-Crystallin Subunits
Soluble crystallins were fractionated using a 2.5 x 95-cm column (Sephacryl S-300 HR; Amersham Pharmacia Biotech, Piscataway, NJ) maintained at 4°C. The mobile phase buffer contained 20 mM Tris (pH 7.5), 1.0 mM EGTA, and 100 mM NaCl and flowed at 25 mL/h. Collected peaks of -, ßH-, ßL-, and -crystallins were then concentrated and desalted by ultrafiltration (YM10 membranes; Millipore, Bedford, MA) and dried by vacuum centrifugation. Individual ßH-crystallin subunits were isolated by anion-exchange HPLC using a 7.5 x 75-mm diethylaminoethyl (DEAE) column (5-PW; TosoHaas, Montgomeryville, PA). Before chromatography, ßH-crystallin aggregates were denatured and reduced by dissolving in 6 M urea, 10 mM Tris (pH 8.5), 50 mM dithiothreitol (DTT), and incubation at 37°C for 30 minutes. The DEAE column mobile phase contained 6 M urea, 10 mM Tris (pH 8.5), and 2 mM DTT at a 1-mL/min flow rate. Three to 10 mg ßH was injected, and after a 15-minute wash, ß-subunits were eluted with a 0- to 80-mM NaCl gradient over 100 minutes.

Measurement of Crystallin Subunit Masses
Approximate 5-µg samples of whole -crystallin aggregate or isolated ß-crystallin subunits were injected onto a 0.5 x 150-mm column (C18 Targa; Higgins Analytical, Mountain View, CA), and masses were determined by on-line analysis of eluents by electrospray ionization mass spectrometry (ESIMS) on an iontrap system (model LCQ; ThermoFinnigan, San Jose, CA). The column used a 10-µL/min flow rate and linear gradient of 10% to 75% acetonitrile over 40 minutes in a mobile phase containing 0.1% acetic acid. Mass spectra of proteins eluting from the C18 column were deconvoluted by computer (Xcalibur software with BioWorks; ThermoFinnigan). Mass accuracy of better than 0.02% was confirmed, using horse myoglobin.

Confirmation of ß-Crystallin Sequences
DEAE-purified ßB3, ßA3, ßA4, and ßB1 were incubated with 10 mM DTT at 37°C for 30 minutes in 6 M urea and then alkylated by addition of 20 mM iodoacetamide at room temperature for 15 minutes. Proteins were then dialyzed to remove urea, and each protein was digested overnight with trypsin, gluC, or aspN proteases, under the conditions recommended by the manufacturer (Roche Molecular Biochemicals). Peptide digests were then analyzed by ESIMS, using the same column and instrument described earlier, except with a linear 7.5% to 37% acetonitrile gradient over 50 minutes. Mass spectra were collected during the liquid chromatography run using a data-dependent "triple-play" strategy. This consisted of a full mass scan (m/z 300-2000), zoom scan on the most abundant ion to determine charge state, and a tandem mass spectrometry (MS/MS) scan to collect collision-induced dissociation (CID) spectra on peptides. Automated analysis of CID spectra to determine the amino acid sequence of peptides was performed on computer (SEQUEST software; ThermoFinnigan) as described by Yates et al.²⁰ A static modification of 57.1 mass units was added to the cysteine mass to account for the addition of the carboxyamido group during alkylation. Confirmation of peptide identification by computer (SEQUEST) was performed by visual inspection of spectra to determine whether continuous strings of matching y and b ions were present above background.

2-DE and Identification of Rat Lens Crystallins
Immobilized pH gradient (IPG) gel strips (18 cm, pH 5–9) were produced using a composition recommended by the manufacturer (Immobiline II; Amersham Pharmacia Biotech). A detailed protocol for pouring IPG gels can be found at a Web site maintained by Angelika Görg at the Technical University of Munich (http://www.edv.agrar.tu-muenchen.de/blm/deg/manual/manfrm.htm). Dried 3-mm wide IPG strips were rehydrated overnight in a reswelling tray (Immobiline DryStrip; Amersham Pharmacia Biotech), as recommended by the manufacturer. The 0.4-mL reswelling solution for each gel contained 8.1 M deionized urea, 2% 3-([3-cholamidopropyl]dimethylammonio)-2-hydroxy-1-propanesulfonate (CHAPS) detergent, 50 mM DTT, 2% IPG buffer (pH 6–11), a trace of bromophenol blue tracking dye, and 400 µg soluble lens proteins from 12-day-old rats. Isoelectric focusing was performed on an electrophoresis apparatus (Multiphor II; Amersham Pharmacia Biotech) using a program of 500 to 3500 V over 1.5 hours, and 3500 V for 12 hours, at a temperature of 35°C.

IPG strips were prepared for the second dimension by two sequential 15-minute incubations in 6 M urea, 50 mM Tris (pH 8.8), 30% glycerol, 2% SDS, and 0.001% bromophenol blue containing, alternately, 2% DTT and 2.5% iodoacetamide. The second-dimension separation was then performed on 24 x 18.5 cm 12% SDS-PAGE gels (IsoDalt; Amersham Pharmacia Biotech). Gels used for image analysis were stained using Coomassie blue G-250,²¹ and gels used for in-gel digestion of proteins were negatively stained with imidazole-zinc.²²

Gel images were analyzed by computer (Melanie 3 software; GeneBio, Geneva, Switzerland). The grid showing the pH of the first-dimension IPG gels and relative molecular weight of the second-dimension gels were determined by computer (Melanie 3) using the calculated pIs of A (5.52), ßB3 (6.83), and C (7.52) and position of low-molecular-weight SDS-PAGE standards (Bio-Rad, Hercules, CA). The calculation of protein pIs was performed on computer (GeneWorks 2.5 software; Oxford Molecular, Campbell, CA), taking into account whether the protein was N acetylated. The assignment of pH on the IPG gels was validated by comparison with an internal standard of carbamylated rabbit muscle glyceraldehyde-3-phosphate dehydrogenase (GAPDH; G-5262; Sigma, St. Louis, MO) produced using the method of Link.²³ The pIs of the various carbamylated species were determined by sequentially removing lysines from the sequence of GAPDH before calculation of pIs. The estimated pIs of crystallins differed by less than 0.15 pH units between the two methods.

Crystallin subunits were identified on 2-DE gels by MS. Negatively stained spots from one to three 2-DE gels of soluble protein from 12-day-old lenses were manually excised, washed, and dried and proteins within gel slices digested using sequencing grade–modified trypsin (Promega, Madison, WI), as previously described.²⁴ Crystallins were then identified by on-line ESIMS analysis of peptides as described earlier (SEQUEST software; ThermoFinnigan) for interpretation of MS/MS spectra.

	Results

Top Abstract Introduction Methods Results Discussion References

 
Before this study, the entire sequence of rat ßA4 and N-terminal sequence of rat ßA3 were unknown. The complete cDNA sequence of rat ßA4 was determined by a combination of 3' and 5'RACE PCR. The resultant 800-bp sequence (GenBank accession no. AF013247; Fig. 1A ) encoded a protein 195 amino acids in length, because of the removal of the N-terminal methionine in the mature protein. The cDNA for rat ßA3 was similarly amplified by 5'RACE PCR to yield a 161-bp sequence (GenBank accession no. AF013248) encoding the N-terminal 52-amino-acid residues of the protein, 38 of which were previously unreported (Fig. 1B) .²⁵ ßA3 is the only rat ß-crystallin that retains its N-terminal methionine in the mature protein. This 5' sequence also contained the alternate start codon that yields ßA1, a protein identical with ßA3, except there are 18 fewer amino acids at its N terminus.

View larger version (47K): [in this window] [in a new window]   Figure 1. cDNA and deduced amino acid sequences for four rat ß-crystallins that were either previously unknown or that had sequences that were inconsistent with their measured masses. (A) ßA4 cDNA and deduced protein sequence (GenBank accession no. AF013247). The polyadenylation signal is underscored. (B) ßA3 cDNA 5' sequence. Only the first 119 nucleotides of the 161-bp sequence (GenBank accession no. AF013248) are shown. Nucleotides 6-119 code for the 38 N-terminal amino acid residues that were previously unknown. The alternate start codon producing ßA1 crystallin is underscored. (C) ßB1 cDNA and deduced protein sequence. Only 39 bp of the 741-bp sequence (GenBank accession no. AF286652) are shown (nucleotides 31-69). This region contained three nucleotides (underscored) differing from the previously published sequence, whereas the remaining nucleotides not shown were identical. The amino acids that differ from the earlier sequence are underscored. Numbering was initiated on the first nucleotide of the start codon. (D) ßB3 cDNA 5' sequence. Only 300 bp of the 660-bp sequence (GenBank accession no. X05899) containing differences from the earlier sequence are shown. Underscored nucleotides that differed from the previous sequence resulted in the change of three amino acids (underscored). Nucleotide 138 contained a T-C polymorphism (Fig. 2) resulting in either leucine or serine at residue 41 in the protein (denoted as X). N-terminal methionines were not included in the deduced protein sequences of ßA4, ßB1, and ßB3 because they are removed from the mature protein (see Fig. 5 ).

An amplified 660-bp cDNA coding for rat ßB3 was also sequenced (GenBank accession no. AF287304) and compared with the previous cDNA sequence (GenBank accession no. X05899). A difference in nucleotide 54 in the new sequence resulted in a change in amino acid 13 from N to S (Fig. 1D) . This difference was also previously detected by Edman sequencing.²⁶ Direct sequencing of the ßB3 PCR product also resulted in the detection of a polymorphism at nucleotide 138 (Fig. 2) . Both nucleotides T and C were detected at this position, leading to either S or L at amino acid 41 (Fig. 1D) . An additional difference was also found at nucleotides 275-277, resulting in the alteration of amino acid 87 from A to R.

View larger version (20K): [in this window] [in a new window]   Figure 2. (A) Sense and (B) antisense sequences for nucleotides 135-142 of the cDNA for rat ßB3-crystallin as determined by direct sequencing. The presence of both T and C in the sense strand and A and G in the antisense strand at nucleotide 138 indicates a polymorphism at this position.

View larger version (31K): [in this window] [in a new window]   Figure 3. (A) Separation of individual rat ß-crystallin subunits from denatured ßH-crystallin aggregates using DEAE anion-exchange chromatography. The identification of the various peaks was performed by MS analysis of whole proteins and peptides from tryptic digests. (B) SDS-PAGE of purified ß-crystallin subunits from peaks labeled in (A). ßA3 (12-215) denotes the modified ßA3 species missing 11 residues from its N terminus.

View this table: [in this window] [in a new window]   Table 1. Comparison of Calculated and Measured Masses of Isolated Rat and ß-Crystallins

View larger version (16K): [in this window] [in a new window]   Figure 4. ESIMS measurement of isolated rat ßB3 crystallin. The peak at 24,245.7 corresponds to ßB3 with serine at residue 41, whereas the mass at 24,271.5 corresponds to ßB3 with leucine at residue 41. The alteration producing the species at 24,314.2 is unknown.

View larger version (52K): [in this window] [in a new window]   Figure 5. Confirmation of rat ßB1 (A), ßB3 (B), ßA3 (C), and ßA4 (D) sequences by MS/MS analysis of protein digests using trypsin, GluC, and AspN proteases. Peptides covering the entire sequence of each protein were confirmed by MS/MS, including the underscored sequences that differed from previously reported sequences in ßB1 and ßB3. Numbers above each bracketed sequence are the calculated monoisotopic mass for each recovered peptide confirmed by MS/MS. The mass of each cysteine residue was increased by 57.1 because of the alkylation with iodoacetamide. All proteins were N acetylated, and, with the exception of ßA3, all N-terminal methionines were removed. The polymorphic residue 41 of ßB3 containing either serine or leucine was also confirmed by MS/MS (Fig. 6) .

View larger version (29K): [in this window] [in a new window]   Figure 6. Representative MS/MS spectra of tryptic peptide 37-54 of rat ßB3. Spectrum of the peptide containing (A) a serine and (B) a leucine at residue 41. Measured masses of identified y ions (loss of residues at the N terminus) and b ions (loss of residues at the C terminus) are labeled in each spectrum. For comparison, the calculated masses for all observed y and b ions are indicated in the sequence above each spectrum.

To further analyze the crystallin proteome of rat, soluble proteins from the lenses of 16-day-old animals were separated by 2-DE (Fig. 7A) . The identities of the various crystallin subunits on the 2-DE gels were then determined by analysis of between 30% and 90% of each protein’s sequence by MS/MS of peptides (Fig. 7B) . The analysis identified all known rat crystallin subunits, including previously unreported ßA2 and for the first time resolved S from a truncated form of ßA3 missing 11 residues from its N terminus (ßA3_12-215). The comigration of ßA3_12-215 and S on 2-DE gels may have led to the overestimation of the abundance of these two species in earlier work.^{26 28} Because the sequences of rat ßA2 and S remain unknown, the identities of these proteins were determined based on identification of several peptides with sequences that are identical with the published sequences of bovine ßA2 and S (Swiss Prot P26444 and P06504).

View larger version (51K): [in this window] [in a new window]   Figure 7. 2-DE gel showing the proteome map of total soluble protein from lenses of 16-day-old rat. (A) Gel with no labels to facilitate visualization of crystallin spots. Left: molecular weight of protein standards. (B) Gel with labeled identities for each crystallin subunit determined by in-gel digestion and MS/MS analysis. Identities of spots 1 to 4 are not given, because they contained poorly focused -crystallins. The grids showing the molecular weights and pH ranges on the gel were determined as described in the methods section. The regions used to calculate the volume of each protein are shown by the outline surrounding each spot. The percentage volume (relative abundance) of each crystallin subunit is indicated in Figure 8 .

Unlike mouse ßA1 and A_insert,¹ rat ßA1 and A_insert did not resolve from one another during 2-DE. A_insert (Swiss Prot P24623) is identical with A, except for an insertion of 23 extra amino acids because of differential splicing. The identification of A_insert was based on analysis of peptides common to both A_insert and A. Peptides from the unique 23-amino-acid region of A_insert were not recovered from the gel digest. However, because of its much higher relative molecular weight on the gel compared with A, the protein was most likely A_insert, rather than a modified form of A.

A faint spot just below ßB1 was identified as an acidic form of ßB3. The alteration causing this acidification of ßB3 remains unknown. The acidification was not due to proteolysis, because MS analysis indicated that the N and C termini of the protein remained intact (data not shown). This minor species could be the result of an as yet unidentified additional polymorphism in rat ßB3, possibly corresponding to the unknown form of ßB3 with a mass of 24,314 in Figure 4 . By coincidence, this acidic form of rat ßB3 migrated to an identical position after 2-DE as the major form of mouse ßB3.¹

Because of their high sequence homology, the six A–F crystallins were difficult to fully resolve and identify by 2-DE. For example, there are only four amino acid differences between the reported sequences of E and F (Swiss Prot P02528 and P10068, respectively). The proximity of the -crystallin spots also caused some contamination of one protein with another during MS/MS analysis of peptides. This required confirmation that the peptide unique to each protein caused a major ion peak during the reversed-phase separation of the digests. The identification of the -crystallins in this study confirmed the earlier assignments made by Voorter et al.²⁸ The additional species marked with numbers 1 to 4 adjacent to A–F-crystallins were composed of poorly focused A–F crystallins that migrated to more acidic positions than the major forms of A–F. The cause of these additional -species on the 2-DE gels is unknown. Similar acidic forms of -crystallins were also observed on 2-DE gels of mouse lens crystallins.¹

Image analysis was used to estimate the pI and percentage of each crystallin subunit in the soluble proteins from 12-day-old rats. When the calculated pIs of A, ßB3, and C were used to calibrate the pH of the IPG strips, the measured pIs of the other crystallins fell within 0.2 pH units of their calculated values. The reproducibility of the IPG gels resulted in an SD of pI estimation of less than 0.02 pH units. Calculation of mean percentage volumes of spots from multiple 2-DE gels prepared from different rats of identical age allowed simple estimation of the abundance of each crystallin (Fig. 8) . Monomeric -crystallins comprised approximately 60% of the soluble protein of young rat lens, ß-crystallins 25%, and -crystallins 15% (Fig. 8) .

View larger version (15K): [in this window] [in a new window]   Figure 8. The relative abundance of individual crystallins in the lenses of 16-day-old rats. Soluble protein from single pairs of lenses from littermate rats were separated by 2-DE, stained with Coomassie blue, and quantified on computer by image analysis. The percentage volume, calculated from the number and gray-scale value of pixels within a detected spot, was used to estimate the percentage abundance of each crystallin subunit in the lens. Regions 1 to 4 (as labeled in Fig. 7 ) contained poorly focused -crystallins that were included in the analysis to prevent underestimation of the total -crystallin content. The error bars indicate +1 SD (n = 4 gels). Each gel contained 400 µg protein from a single pair of lenses from one rat.

	Discussion

Top Abstract Introduction Methods Results Discussion References

These data extend earlier work in our laboratory, in which the age-related alterations of rat crystallins were examined in both the water-soluble and -insoluble fractions of the lens nucleus and cortex by 2-DE.²⁶ The previous studies documented extensive partial proteolysis of - and ß-crystallins in the water-insoluble fraction of rat lens nucleus during maturation and cataract. The confirmed sequences of the crystallins determined in this study will now allow a more detailed analysis of these proteolyzed crystallins by MS.

The IPG-based 2-DE map of rat crystallins shown in Figure 7 is more detailed than previously available maps.^{28 29} This map for the first time identifies ßA2-crystallin in rat lens, demonstrates comigrating ßA1 and A_insert, resolves the truncation product of ßA3 (ßA3_12-215) from S-crystallin, and allows quantification of the relative amounts of these proteins. The quantification of crystallin subunits in 16-day-old rat lens provides several interesting contrasts when compared with approximately 1-week-old human lens. First, rat lens contained approximately one half the amount of -crystallins found in young human lens.¹⁸ This lower amount of -crystallin may correlate with the shorter life span of rodents and diminished requirement for chaperoning of damaged lens proteins accumulating with age. Second, the percentage of -crystallins in young rat lens is approximately twice that in young human lens. Whereas rat lenses contain all seven -crystallin subunits, human lenses contain only C, D, and S.¹⁸ Furthermore, S-crystallin, the concentration of which rapidly increases with age in rat,²⁸ never reached the concentration found in human, where it becomes a major component of adult lens.¹⁸

Additionally, the subunit composition of ß-crystallins in rat lens was dramatically different from that in human lens. ßB3-crystallin, which comprised nearly 10% of the rat lens soluble protein, is largely undetectable in human lens after birth.¹⁸ In contrast, ßB2 was more than three times as abundant in young human lens than in young rat lens. Crystallins in human lens remain water soluble far into adulthood,³⁰ whereas more than 50% of crystallins of the rat lens nucleus are insoluble by 4 months of age.²⁶ We hypothesize that the high ßB2-to-ßB3 ratio is partially responsible for this increased solubility of crystallins in mature human lens. The high percentage of ßB3 in rat lens may drive protein insolubilization, because it more readily precipitates after partial proteolysis than do other ß-crystallin subunits.²⁹ In contrast, ßB2 is resistant to precipitation, both after partial proteolysis in vitro²⁹ and during aging in human lens.³¹

Detection of a polymorphism in rat ßB3 suggests that polymorphisms may exist in the crystallins of other species as well. A similar study of bovine crystallins detected a polymorphism in bovine ßA3 crystallin (David L, unpublished results, 2001). Previously unknown polymorphisms may also be present in human lens crystallins. These polymorphisms may remain undetected, because of the limited amount of redundant sequencing of human crystallin genes and rapid posttranslational modification of human crystallins with age. Certain polymorphisms in human crystallins may have the potential of increasing the risk of cataract. The ability of mutations in major lens proteins to cause congenital cataracts in humans has been well documented.^{32 33 34}

In conclusion, the results in this study provide baseline data on the composition and primary structure of crystallins in normal rat lens. The information will be useful in future studies to more thoroughly examine both age-related and cataract-specific modifications in rat crystallins. This analysis is important, because similar modifications may be a cause of human cataract.

	Acknowledgements

 
The authors thank Jean Smith and David Smith, University of Nebraska, and Margaret Sheil, Greg Kilby, and John Carver, University of Wollongong, New South Wales, Australia, for performing the initial measurements of rat crystallin masses that began this study.

	Footnotes

 
³ Present affiliation: TRA Urology Research Center, Bayer Yakuhin Ltd., Kyoto, Japan.

Supported by National Eye Institute Grants EY-07755 and EY-12016 (LLD), EY-12239 (KJL), and EY-03600 (TRS).

Submitted for publication April 27, 2001; accepted June 27, 2001.

Commercial relationships policy: N.

The publication costs of this article were defrayed in part by page charge payment. This article must therefore be marked "advertisement" in accordance with 18 U.S.C. 1734 solely to indicate this fact.

Corresponding author: Larry L. David, School of Dentistry, Department of Oral Molecular Biology, Oregon Health & Science University, 611 SW Campus Drive, Portland, OR 97201; davidl{at}ohsu.edu.

	References

Top Abstract Introduction Methods Results Discussion References

 

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