Srivastava O P, Srivastava K
Department of Physiological Optics, University of Alabama at Birmingham 35294, USA.
Exp Eye Res. 1996 Jun;62(6):593-604. doi: 10.1006/exer.1996.0070.
The purpose of this study was to determine whether a 9 kDa gamma D-crystallin fragment, on in vivo post-translational modifications, exists as isoforms in the water soluble protein fraction of human lenses. In this study, three isoforms of the 9 kDa polypeptide (named as 9 kDa I, II and III) were identified and purified. In addition, the possible modified amino acids and their locations in the three isoforms were identified. The purification of the three isoforms was achieved by four steps which included separation of a mixture of crystallin fragments from the intact crystallins by a Sephadex G-50 chromatography under denaturing conditions, followed by purification of the 9 kDa polypeptide isoforms by a non-denaturing gel electrophoresis, preparative SDS-PAGE and HPLC using a C-18 column. Each of the isoforms showed a single protein band and a single peak during SDS-PAGE and HPLC analyses respectively. The three isoforms on their partial N-terminal sequence analyses, exhibited sequence identical to gamma D-crystallin starting at residue no. 87 suggesting that the isoforms contained residues no. 87 to 173 of gamma D-crystallin. On comparison of the amino acid compositions of the isoforms with that of the identical 9 kDa gamma D-crystallin fragment, the isoforms showed relatively lower amino contents of Asp, Arg, Leu and Tyr residues suggesting modifications of these residues in the isoforms. To identify the specific regions at which these amino acid residues were modified, the Western blot analysis with six site-specific polyclonal antibodies to six regions of the 9 kDa gamma D-crystallin polypeptide was carried out. Of the six antibodies raised, one was to the N-terminal region (residue nos 87-95; named as anti-9 kDa N-Ab), second to the C-terminal region (residue nos 165-173; named as anti-9 kDa C-Ab) and four to the four different middle regions [named as anti-9 kDa M1 (nos 94-100)-Ab, M2 (nos 114-120)-Ab, M3 (nos 137-143)-Ab and M4 (nos 149-154)-Ab] of the polypeptide. The Western blot analysis suggested that the 9 kDa I and 9 kDa II isoforms had modified amino acid residues in the regions of residue nos 114-120 and 165-173 whereas the 9 kDa III isoform in the regions of residue nos 114-120, 137-143, 149-154 and 165-173. It was also determined whether the 9 kDa isoforms exhibit an age-related appearance in human lenses. Western blot analysis as above of the WS-proteins from lenses from donors of different ages was carried out. On comparison of these results with an identical Western blot analysis of the three purified 9 kDa isoforms, I, II and III, it was inferred that the 9 kDa isoform III appeared earlier than other isoforms during aging in human lenses.
本研究的目的是确定一种9 kDa的γD-晶状体蛋白片段在体内进行翻译后修饰后,是否以异构体形式存在于人晶状体的水溶性蛋白组分中。在本研究中,鉴定并纯化了9 kDa多肽的三种异构体(命名为9 kDa I、II和III)。此外,还鉴定了三种异构体中可能发生修饰的氨基酸及其位置。通过四个步骤实现了三种异构体的纯化,包括在变性条件下通过Sephadex G-50色谱从完整晶状体蛋白中分离晶状体蛋白片段混合物,随后通过非变性凝胶电泳、制备性SDS-PAGE和使用C-18柱的HPLC纯化9 kDa多肽异构体。在SDS-PAGE和HPLC分析中,每种异构体分别显示出一条单一的蛋白条带和一个单一的峰。对三种异构体进行部分N端序列分析时,发现其序列与γD-晶状体蛋白从第87位残基开始相同,这表明这些异构体包含γD-晶状体蛋白的第87至173位残基。将异构体的氨基酸组成与相同的9 kDaγD-晶状体蛋白片段的氨基酸组成进行比较时,异构体显示出Asp、Arg、Leu和Tyr残基的氨基酸含量相对较低,这表明这些残基在异构体中发生了修饰。为了确定这些氨基酸残基发生修饰的具体区域,使用针对9 kDaγD-晶状体蛋白多肽六个区域的六种位点特异性多克隆抗体进行了蛋白质印迹分析。在产生的六种抗体中,一种针对N端区域(第87 - 95位残基;命名为抗9 kDa N-Ab),第二种针对C端区域(第165 - 173位残基;命名为抗9 kDa C-Ab),另外四种针对多肽的四个不同中间区域[命名为抗9 kDa M1(第94 - 100位)-Ab、M2(第114 - 120位)-Ab、M3(第137 - 143位)-Ab和M4(第149 - 154位)-Ab]。蛋白质印迹分析表明,9 kDa I和9 kDa II异构体在第114 - 120位和第165 - 173位残基区域有修饰的氨基酸残基,而9 kDa III异构体在第114 - 120位、第137 - 143位、第149 - 154位和第165 - 173位残基区域有修饰。还确定了9 kDa异构体在人晶状体中是否呈现与年龄相关的出现情况。对来自不同年龄供体晶状体的WS-蛋白进行了上述蛋白质印迹分析。将这些结果与对三种纯化的9 kDa异构体I、II和III进行的相同蛋白质印迹分析结果进行比较时,推断出在人晶状体老化过程中,9 kDa异构体III比其他异构体出现得更早。
