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人腺癌/上皮细胞表面抗原互补DNA的分子克隆与特性分析

Molecular cloning and characterization of a human adenocarcinoma/epithelial cell surface antigen complementary DNA.

作者信息

Strnad J, Hamilton A E, Beavers L S, Gamboa G C, Apelgren L D, Taber L D, Sportsman J R, Bumol T F, Sharp J D, Gadski R A

机构信息

Lilly Research Laboratories, Eli Lilly and Company, Indianapolis, Indiana 46285.

出版信息

Cancer Res. 1989 Jan 15;49(2):314-7.

PMID:2463074
Abstract

A human adenocarcinoma-associated antigen (KSA) defined by the monoclonal antibody KS1/4 has become the focus of several site-directed strategies for tumor therapy. KSA, a 40,000 Da cell surface glycoprotein antigen, is found at a high density in all adenocarcinomas examined to date and in corresponding normal epithelial tissues. Here we describe the cloning and sequencing of overlapping complementary DNA clones which encode the entire KSA as expressed in UCLA-P3, a human lung adenocarcinoma cell line. We have deduced the 314-amino acid sequence and have compared it to the N-terminal amino acid sequence data of the affinity-purified antigen. The KSA is synthesized as a 314-residue-long preproprotein that is then processed to a 232-residue-long antigen. KSA appears to have a single transmembrane domain of 23 residues that separates the highly charged 26-residue cytoplasmic domain from the extracellular domain. The N-terminal region of the propeptide is rich in cysteines and contains three potential N-glycosylation sites. Computer-assisted analyses at both the DNA and protein levels have found no significant similarities of this protein to known sequences, but a GC-rich 5' terminus is evident. Northern blot analysis shows that transcription of KSA can be detected in RNA isolated from normal colon but not in RNA isolated from normal lung, prostate, or liver.

摘要

一种由单克隆抗体KS1/4定义的人腺癌相关抗原(KSA)已成为多种肿瘤治疗定点策略的焦点。KSA是一种40000道尔顿的细胞表面糖蛋白抗原,在迄今为止检测的所有腺癌以及相应的正常上皮组织中都以高密度存在。在此,我们描述了重叠互补DNA克隆的克隆和测序,这些克隆编码了在人肺腺癌细胞系UCLA-P3中表达的完整KSA。我们推导了314个氨基酸的序列,并将其与亲和纯化抗原的N端氨基酸序列数据进行了比较。KSA最初合成的前体蛋白有314个残基,随后加工成有232个残基的抗原。KSA似乎有一个由23个残基组成的单一跨膜结构域,将带高电荷的26个残基的胞质结构域与胞外结构域分隔开。前肽的N端区域富含半胱氨酸,并含有三个潜在的N糖基化位点。在DNA和蛋白质水平上的计算机辅助分析均未发现该蛋白与已知序列有明显相似性,但5'端富含GC。Northern印迹分析表明,在从正常结肠分离的RNA中可检测到KSA的转录,但在从正常肺、前列腺或肝脏分离的RNA中未检测到。

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