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转染卡波西肉瘤DNA后重排的人转化基因的分离

Isolation of a rearranged human transforming gene following transfection of Kaposi sarcoma DNA.

作者信息

Delli Bovi P, Basilico C

出版信息

Proc Natl Acad Sci U S A. 1987 Aug;84(16):5660-4. doi: 10.1073/pnas.84.16.5660.

Abstract

By transfecting high molecular weight DNA from a Kaposi sarcoma lesion into murine NIH 3T3 cells, we have identified and molecularly cloned a set of human DNA sequences capable of inducing focus formation, growth in agar, and tumorigenicity in these cells. The human DNA sequences present in primary, secondary, and tertiary NIH 3T3 transformants encompass about 32 kilobases (kb) and contain four rearrangements with respect to normal human DNA and a portion of the c-fms protooncogene (FMS in human gene nomenclature). However, the minimal transforming region (6.6 kb) identified in our cloned DNA borders on the c-fms DNA region but does not contain c-fms coding sequences. The fms sequences are also not represented in the two transcripts (approximately equal to 1.2 and 3.5 kb) detected in NIH 3T3 transformants; however, they might provide elements regulating expression. Hybridization to several known oncogene probes and preliminary sequencing data indicate that we have identified a previously unrecognized "activated" oncogene. Since the rearrangements present in our cloned DNA sequences are not detectable in the original Kaposi tumor DNA used for transfection, it is possible that this oncogene was generated during gene transfer.

摘要

通过将来自卡波西肉瘤病变的高分子量DNA转染到小鼠NIH 3T3细胞中,我们已经鉴定并分子克隆了一组能够在这些细胞中诱导集落形成、在软琼脂中生长以及致瘤性的人类DNA序列。存在于原代、二代和三代NIH 3T3转化体中的人类DNA序列约为32千碱基(kb),并且相对于正常人类DNA和部分c-fms原癌基因(人类基因命名法中的FMS)包含四处重排。然而,我们在克隆DNA中鉴定出的最小转化区域(6.6 kb)毗邻c-fms DNA区域,但不包含c-fms编码序列。fms序列在NIH 3T3转化体中检测到的两种转录本(约1.2和3.5 kb)中也未出现;不过,它们可能提供调控表达的元件。与几种已知癌基因探针的杂交以及初步测序数据表明,我们已经鉴定出一种先前未被识别的“激活的”癌基因。由于在用于转染的原始卡波西肿瘤DNA中检测不到我们克隆的DNA序列中存在的重排,所以这种癌基因有可能是在基因转移过程中产生的。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5e02/298922/cba31f871960/pnas00331-0161-a.jpg

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