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src家族cDNA的比较揭示了转染成纤维细胞中集落形成的不同机制。

Comparison of src-family cDNAs reveals distinct mechanisms underlying focus formation in transfected fibroblasts.

作者信息

Sartor O, McLellan C A, Chiueh T

机构信息

Clinical Pharmacology Branch, National Cancer Institute, Bethesda, Maryland 20892.

出版信息

J Biol Chem. 1992 Oct 15;267(29):21044-51.

PMID:1383216
Abstract

Despite the intensive study of both cellular transformation and src-family protein-tyrosine kinases, there have been no direct comparisons of transforming potency for normal members of this gene-family. In this study, the focus-forming activity of normal c-src, fyn, and lck cDNAs were compared in NIH 3T3 cell transfection assays. Focus formation was studied quantitatively, and individual foci were analyzed for phosphotyrosine content and expression of appropriate translational products. Each foci arising from c-src transfectants had a marked increase in phosphotyrosine content, and the majority of these foci expressed a c-src protein with an aberrant carboxyl terminus. Foci derived from lck transfectants also had a marked increase in phosphotyrosine content, and some foci expressed a lck protein with an aberrant carboxyl terminus. In contrast, foci from fyn-transfected cells were not distinguished from G418-selected mass cultures in terms of total phosphotyrosine content or expression of p59fyn. These studies support the previously published concept that overexpression of the normal fyn protein contributes to focus formation in transfected NIH 3T3 cells but suggest that the focus-forming activity observed after c-src or lck transfections is frequently attributable to mutational events. Because lck mutations have not been previously described in transformed foci, we characterized the lck transcript expressed in two foci and identified a novel point mutation that encodes a lck protein with increased in vivo kinase and focus-forming activity.

摘要

尽管对细胞转化和src家族蛋白酪氨酸激酶都进行了深入研究,但尚未对该基因家族正常成员的转化能力进行直接比较。在本研究中,我们在NIH 3T3细胞转染试验中比较了正常c-src、fyn和lck cDNA的集落形成活性。对集落形成进行了定量研究,并对单个集落的磷酸酪氨酸含量和相应翻译产物的表达进行了分析。来自c-src转染子的每个集落的磷酸酪氨酸含量都有显著增加,并且这些集落中的大多数都表达了一种羧基末端异常的c-src蛋白。来自lck转染子的集落的磷酸酪氨酸含量也有显著增加,并且一些集落表达了一种羧基末端异常的lck蛋白。相比之下,就总磷酸酪氨酸含量或p59fyn的表达而言,来自fyn转染细胞的集落与G418选择的大量培养物没有区别。这些研究支持了先前发表的观点,即正常fyn蛋白的过表达有助于转染的NIH 3T3细胞中的集落形成,但表明在c-src或lck转染后观察到的集落形成活性通常归因于突变事件。由于以前在转化集落中未描述过lck突变,我们对在两个集落中表达的lck转录本进行了表征,并鉴定了一个新的点突变,该突变编码一种体内激酶活性和集落形成活性增加的lck蛋白。

相似文献

1
Comparison of src-family cDNAs reveals distinct mechanisms underlying focus formation in transfected fibroblasts.src家族cDNA的比较揭示了转染成纤维细胞中集落形成的不同机制。
J Biol Chem. 1992 Oct 15;267(29):21044-51.
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v-src mutations outside the carboxyl-coding region are not sufficient to fully activate transformation by pp60c-src in NIH 3T3 cells.羧基编码区域以外的v-src突变不足以在NIH 3T3细胞中通过pp60c-src完全激活转化。
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