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维甲酸可下调人乳腺癌细胞系中1型血管活性肠肽受体的表达。

Retinoic acid down-regulates the expression of the vasoactive intestinal polypeptide receptor type-1 in human breast carcinoma cell lines.

作者信息

Madsen B, Georg B, Vissing H, Fahrenkrug J

机构信息

Department of Clinical Biochemistry, Bispebjerg University Hospital, Copenhagen, Denmark.

出版信息

Cancer Res. 1998 Nov 1;58(21):4845-50.

PMID:9809989
Abstract

Four breast carcinoma cell lines (T47D, ZR-75-1, MDA-MB-231, and MCF-7) were tested for regulation of the expression of vasoactive intestinal polypeptide receptor type-1 (VIP-R1). In all four cell lines, retinoic acid (RA) treatment caused a fast and marked decrease in VIP-R1 mRNA level as examined by Northern blots. Cycloheximide pretreatment attenuated the effect from 3- to 2-fold, indicating that existing proteins can mediate the decreasing effect of RA, but to attain the maximal effect new protein synthesis might be needed. Transcriptional inhibition with Actinomyocin D showed that RA did not influence the VIP-R1 mRNA half-life, indicating that the decreasing effect of RA on the mRNA level is due to transcriptional inhibition. In agreement with the observations on mRNA level, we found that the VIP receptor number was reduced 3-fold from 88 to 32 fmol/10(6) cells in T47D cells and from 222 to 73 fmol/10(6) cells in MDA-MB-231 cells upon RA treatment for 72 h. The promoter and 5'-flanking region of the VIP-R1 gene were cloned from a human placental cosmid library, and 2.5 kb were sequenced to search for regulatory elements. Our results, therefore, imply that the regulation of VIP-R1 gene expression by RA could have a role in human mammary tumor biology.

摘要

对四种乳腺癌细胞系(T47D、ZR - 75 - 1、MDA - MB - 231和MCF - 7)进行了血管活性肠肽1型受体(VIP - R1)表达调控的检测。在所有这四种细胞系中,通过Northern印迹法检测发现,视黄酸(RA)处理导致VIP - R1 mRNA水平快速且显著下降。放线菌酮预处理使该效应减弱至原来的三分之一到二分之一,这表明现有蛋白质可介导RA的降低效应,但要达到最大效应可能需要新的蛋白质合成。用放线菌素D进行转录抑制表明,RA不影响VIP - R1 mRNA的半衰期,这表明RA对mRNA水平的降低效应是由于转录抑制。与mRNA水平的观察结果一致,我们发现,在RA处理72小时后,T47D细胞中的VIP受体数量从88 fmol/10⁶细胞减少到32 fmol/10⁶细胞,MDA - MB - 231细胞中的VIP受体数量从222 fmol/10⁶细胞减少到73 fmol/10⁶细胞。从人胎盘粘粒文库中克隆了VIP - R1基因的启动子和5'侧翼区域,并对2.5 kb进行了测序以寻找调控元件。因此,我们的结果表明,RA对VIP - R1基因表达的调控可能在人类乳腺肿瘤生物学中发挥作用。

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