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β4整合素亚基表达在低转移癌变体中下调。

Beta 4 integrin subunit expression is downregulated in low metastatic carcinoma variants.

作者信息

Cimino L, Perrotti D, D'Agostino G, Falcioni R, Sacchi A

机构信息

Molecular Oncogenesis Laboratory, Regina Elena Cancer Institute, Rome, Italy.

出版信息

Cancer Detect Prev. 1997;21(2):158-66.

PMID:9101077
Abstract

Organization and expression of the gene coding for beta 4 integrin subunit were investigated in murine carcinoma lines endowed with low and high metastatic potential maintained both in vivo and in vitro. Probes corresponding to either the extracellular or the cytoplasmic domains of the protein were generated and employed for Southern and Northern blot hybridization experiments. Southern blot analysis demonstrates a restriction fragment-length polymorphism between BALB/c and C57BI/6J DNAs. The different genomic organization of the beta 4 gene apparently does not generate variation in mRNA length. Northern blot analysis reveals a 7-kb transcript encoding full-length beta 4 protein and shorter transcripts that apparently correspond to nonfunctional mRNAs. In carcinoma cells endowed with low metastatic capacity, the 7-kb mRNA cannot be revealed in spite of the presence of shorter transcripts. In contrast, the 7-kb transcript is always present in tumor cells endowed with high metastatic capacity. Accordingly, the beta 4 protein is detectable, either by immunofluorescence or by Western blot analyses, only in highly metastatic carcinoma cells. In conclusion, the data presented show that in these murine carcinoma cell lines (i) the 7-kb mRNA is associated with a more invasive phenotype, and (ii) missing expression of the beta 4 integrin subunit in low metastatic carcinoma cells depends, at least in part, on mechanisms acting at a post-transcriptional level. The possibility that beta 4 subunit expression is a consequence of specific differentiation stages of lung carcinoma cells is discussed.

摘要

在体内和体外培养的具有低转移潜能和高转移潜能的小鼠癌细胞系中,研究了编码β4整合素亚基的基因的组织和表达情况。制备了与该蛋白的细胞外或细胞质结构域相对应的探针,并用于Southern和Northern印迹杂交实验。Southern印迹分析表明,BALB/c和C57BI/6J DNA之间存在限制性片段长度多态性。β4基因不同的基因组结构显然并未导致mRNA长度的变化。Northern印迹分析显示,有一个7 kb的转录本编码全长β4蛋白,还有一些较短的转录本,显然对应于无功能的mRNA。在转移能力低的癌细胞中,尽管存在较短的转录本,但7 kb的mRNA却无法检测到。相反,在转移能力高的肿瘤细胞中,7 kb的转录本总是存在。因此,只有在高转移癌细胞中,才能通过免疫荧光或Western印迹分析检测到β4蛋白。总之,所提供的数据表明,在这些小鼠癌细胞系中:(i)7 kb的mRNA与更具侵袭性的表型相关;(ii)低转移癌细胞中β4整合素亚基的表达缺失至少部分取决于转录后水平的作用机制。文中还讨论了β4亚基表达是肺癌细胞特定分化阶段结果的可能性。

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