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大鼠多药耐药相关蛋白2基因的克隆与调控

Cloning and regulation of the rat mdr2 gene.

作者信息

Brown P C, Thorgeirsson S S, Silverman J A

机构信息

National Institute of General Medical Sciences, National Institutes of Health, Bethesda, MD 20892.

出版信息

Nucleic Acids Res. 1993 Aug 11;21(16):3885-91. doi: 10.1093/nar/21.16.3885.

Abstract

We have cloned the complete cDNA encoding the rat mdr2 gene by a combination of library screening and the polymerase chain reaction. The sequence of rat mdr2 cDNA is highly similar to other members of the mdr gene family but the initiation of transcription, tissue distribution and regulation of expression of rat mdr2 diverge from the other isoforms. Primer extension analysis showed rat mdr2 mRNA to have a major transcription start point at -277 and a minor one at approximately -518. We constructed gene specific probes for rat mdr2 and mdr1b and compared the expression patterns of these two genes. The highest expression of mdr2 mRNA was in the muscle, heart, liver and spleen. Both mdr2 and 1b mRNA levels were elevated in the livers of rats treated with CCl4 or following partial hepatectomies although the time course of induction of each gene differed. Mdr1b increased by 12 to 24 hours while mdr2 did not increase until 48 hours. Treatment of isolated hepatocytes or RC3 cells with cycloheximide did not effect mdr2 mRNA. In contrast, mdr1b expression was increased. These data suggest that rat mdr2, unlike mdr1b, is not regulated by a negative trans-acting protein factor.

摘要

我们通过文库筛选和聚合酶链反应相结合的方法克隆了编码大鼠多药耐药蛋白2(mdr2)基因的完整cDNA。大鼠mdr2 cDNA的序列与mdr基因家族的其他成员高度相似,但大鼠mdr2的转录起始、组织分布和表达调控与其他异构体不同。引物延伸分析表明,大鼠mdr2 mRNA的主要转录起始点在-277,次要转录起始点在大约-518。我们构建了大鼠mdr2和mdr1b的基因特异性探针,并比较了这两个基因的表达模式。mdr2 mRNA的最高表达出现在肌肉、心脏、肝脏和脾脏中。在用四氯化碳处理的大鼠肝脏或部分肝切除术后,mdr2和mdr1b的mRNA水平均升高,尽管每个基因的诱导时间进程不同。mdr1b在12至24小时增加,而mdr2直到48小时才增加。用环己酰亚胺处理分离的肝细胞或RC3细胞对mdr2 mRNA没有影响。相反,mdr1b的表达增加。这些数据表明,与mdr1b不同,大鼠mdr2不受负性反式作用蛋白因子的调控。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5a7b/309915/83a3f2b51b96/nar00065-0279-a.jpg

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