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肿瘤细胞无法在人脐静脉内皮细胞培养物中反式诱导端粒酶。

Tumor cells fail to trans-induce telomerase in human umbilical vein endothelial cell cultures.

作者信息

Pascale Esterina, Cimino Reale Graziella, D'Ambrosio Ettore

机构信息

Dipartimento di Medicina Sperimentale e Patologia, Università La Sapienza, Roma, Italy.

出版信息

Cancer Res. 2004 Nov 1;64(21):7702-5. doi: 10.1158/0008-5472.CAN-04-1711.

Abstract

The shortening of the telomeres that occurs in most somatic cells and untransformed cell cultures is considered a hallmark of cellular senescence. Re-activation of telomerase, which is usually present in immortal cells, avoids telomere shortening and considerably extends the culture life span. Normal human endothelial cells are characterized by an accelerated rate of telomere shortening and reach replicative senescence after a limited number of cell divisions. It has recently been reported that human telomerase reverse transcriptase expression may be strongly up-regulated in human endothelial cells cocultivated with tumor cells. Due to the important implications of this finding on tumor progression, we have extensively analyzed for the presence of telomerase in primary human endothelial cells either cocultivated with tumor cells or grown with tumor-conditioned medium. We found modest, but readily detectable, amounts of telomerase in all human endothelial cell cultures analyzed that disappeared as the cultures approached senescence. Quantitative reverse transcription-PCR also showed a direct correlation between human telomerase reverse transcriptase expression and the proliferative index of the cultures. Nevertheless, we did not find any evidence of induction of telomerase activity by tumor cells in any of the tested conditions. All data indicate that telomerase in human endothelial cells follows an activation program that is strictly associated to the culture growth rate.

摘要

大多数体细胞和未转化细胞培养物中发生的端粒缩短被认为是细胞衰老的一个标志。端粒酶的重新激活通常存在于永生化细胞中,可避免端粒缩短并显著延长培养物的寿命。正常人内皮细胞的特征是端粒缩短速度加快,在有限数量的细胞分裂后达到复制性衰老。最近有报道称,在与肿瘤细胞共培养的人内皮细胞中,人端粒酶逆转录酶的表达可能会强烈上调。由于这一发现对肿瘤进展具有重要意义,我们广泛分析了与肿瘤细胞共培养或用肿瘤条件培养基培养的原代人内皮细胞中端粒酶的存在情况。我们在所分析的所有人内皮细胞培养物中发现了适量但易于检测到的端粒酶,随着培养物接近衰老,端粒酶消失。定量逆转录聚合酶链反应也显示人端粒酶逆转录酶表达与培养物的增殖指数之间存在直接相关性。然而,在任何测试条件下,我们都没有发现肿瘤细胞诱导端粒酶活性的任何证据。所有数据表明,人内皮细胞中的端粒酶遵循一个与培养物生长速率严格相关的激活程序。

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