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骨桥蛋白-k的cDNA的分离与鉴定:一种与骨桥蛋白具有高度同源性的肾细胞粘附分子。

Isolation and characterization of a cDNA for osteopontin-k: a kidney cell adhesion molecule with high homology to osteopontins.

作者信息

Crivello J F, Delvin E

机构信息

Department of Physiology and Neurobiology, University of Connecticut, Storrs.

出版信息

J Bone Miner Res. 1992 Jun;7(6):693-9. doi: 10.1002/jbmr.5650070614.

Abstract

Screening of a bovine renal cDNA library with MAbs resulted in the isolation of a 1447 bp cDNA. This cDNA (pBk2.1) was sequenced and shown to contain an open reading frame with a putative protein of 261 amino acids, with a molecular weight of 29,573 (minute leader sequence) and a hydrophobic leader sequence of 16 amino acids. pBk2.1 was shown to share a high level of nucleic acid sequence homology over portions of its sequence to human, porcine, mouse, and rat osteopontins (40-60%). The peptide (osteopontin-k) had a potential glycosylation site (Asn-X-Ser/Thr), a GRGDS receptor binding region, a high level of asparagine residues, and a high abundance of acid amino acids characteristic of osteopontin-like cell adhesion molecules. The N-terminal amino acid region of pBk2.1 (the first 82 amino acids) and 42 amino acids at the C terminus had the highest level of homology with the osteopontins at 86%. The middle portion of the peptide had greatly reduced homology, ranging from 50% (amino acids 83-174) to 12% (amino acids 175-219). There were also deletions and additions of sequence in osteopontin-k that were not found in the other osteopontins. The homologies suggest that these proteins are highly related and may be derived from a common gene by alternative splicing. A 678 bp cRNA probe constructed from pBk2.1, containing a region with low homology to the osteopontins (amino acids 183-219 with less than 20% homology, plus amino acids 220-261 and untranslated sequence), was used in northern blots and RNAse protection assays.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

用单克隆抗体筛选牛肾cDNA文库,得到了一个1447bp的cDNA。对该cDNA(pBk2.1)进行测序,结果显示其包含一个开放阅读框,推测编码的蛋白质有261个氨基酸,分子量为29,573(微小前导序列),并有一个16个氨基酸的疏水前导序列。结果表明,pBk2.1在其部分序列上与人、猪、小鼠和大鼠的骨桥蛋白具有较高水平的核酸序列同源性(40%-60%)。该肽(骨桥蛋白-k)有一个潜在的糖基化位点(Asn-X-Ser/Thr)、一个GRGDS受体结合区域、高水平的天冬酰胺残基以及骨桥蛋白样细胞粘附分子特有的高丰度酸性氨基酸。pBk2.1的N端氨基酸区域(前82个氨基酸)和C端的42个氨基酸与骨桥蛋白的同源性最高,为86%。该肽的中间部分同源性大大降低,从50%(氨基酸83-174)到12%(氨基酸175-219)。骨桥蛋白-k中还存在其他骨桥蛋白中未发现的序列缺失和添加。这些同源性表明这些蛋白质高度相关,可能是由一个共同基因通过可变剪接产生的。由pBk2.1构建的一个678bp的cRNA探针,包含一个与骨桥蛋白同源性较低的区域(氨基酸183-219,同源性小于20%,加上氨基酸220-261和非翻译序列),用于Northern印迹和RNA酶保护分析。(摘要截短于250字)

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