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两种针对人骨连接蛋白中心部分的单克隆抗体的表位作图

Epitope mapping of two monoclonal antibodies to the central portion of human osteonectin.

作者信息

Villarreal X C, Malaval L, Mann K G, Delmas P, Long G L

机构信息

Department of Biochemistry, University of Vermont, Burlington 05405.

出版信息

Calcif Tissue Int. 1991 Feb;48(2):138-41. doi: 10.1007/BF02555878.

Abstract

In this study preliminary characterization of two monoclonal antibodies against osteonectin was undertaken. One monoclonal originally raised against bovine bone osteonectin cross reacts with human bone and platelet osteonectin. The other monoclonal antibody has been reported to react with osteonectin derived from human bone and bovine bone but not to the same extent with that from platelets. Initial mapping of the antigenic determinants for both monoclonals was done by testing their ability to bind to the expressed forms of osteonectin in two overlapping SaOS-2 lambda gt11 osteonectin cDNA clones. One clone contains a 0.54 kb insert and is comprised of 50 nucleotides of 5' noncoding and a coding segment for a 17 amino acid signal peptide and 146 amino acids of the N-terminal region of the mature protein. The other clone has a 1.9 kb insert, and includes amino acid no. 18 to the C-terminus of the molecule (amino acid no. 286), a single termination codon, and 1115 nucleotides of 3' noncoding sequence. Both monoclonals recognized expressed osteonectin from the two lambda gt11 SaOS-2 cDNA clones. These results localize the epitope to a region between amino acids 18-146 of osteonectin.

摘要

在本研究中,对两种抗骨连接蛋白的单克隆抗体进行了初步表征。一种最初针对牛骨骨连接蛋白产生的单克隆抗体与人骨和血小板骨连接蛋白发生交叉反应。另一种单克隆抗体据报道可与源自人骨和牛骨的骨连接蛋白发生反应,但与源自血小板的骨连接蛋白反应程度不同。通过测试两种单克隆抗体与两个重叠的SaOS-2 λgt11骨连接蛋白cDNA克隆中表达的骨连接蛋白形式的结合能力,对这两种单克隆抗体的抗原决定簇进行了初步定位。一个克隆包含一个0.54 kb的插入片段,由50个5'非编码核苷酸和一个编码17个氨基酸信号肽以及成熟蛋白N端区域146个氨基酸的编码片段组成。另一个克隆有一个1.9 kb的插入片段,包括分子第18位氨基酸到C端(第286位氨基酸)、一个终止密码子以及1115个3'非编码序列核苷酸。两种单克隆抗体均识别来自两个λgt11 SaOS-2 cDNA克隆的表达的骨连接蛋白。这些结果将表位定位在骨连接蛋白第18 - 146位氨基酸之间的区域。

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