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人类细胞体外PIG-A基因突变试验的开发

Development of an in vitro PIG-A gene mutation assay in human cells.

作者信息

Rees Benjamin J, Tate Matthew, Lynch Anthony M, Thornton Catherine A, Jenkins Gareth J, Walmsley Richard M, Johnson George E

机构信息

Institute of Life Science, Swansea University Medical School, Singleton Park, Swansea SA2 8PP, UK.

Gentronix Ltd BioHub at Alderley Park, Alderley Edge, Cheshire, SK10 4TF, UK.

出版信息

Mutagenesis. 2017 Mar 1;32(2):283-297. doi: 10.1093/mutage/gew059.

Abstract

Mutagens can be carcinogens, and traditionally, they have been identified in vitro using the Salmonella 'Ames' reverse mutation assay. However, prokaryotic DNA packaging, replication and repair systems are mechanistically very different to those in the humans we inevitably seek to protect. Therefore, for many years, mammalian cell line genotoxicity assays that can detect eukaryotic mutagens as well as clastogens and aneugens have been used. The apparent lack of specificity in these largely rodent systems, due partly to their mutant p53 status, has contributed to the use of animal studies to resolve data conflicts. Recently, silencing mutations at the PIG-A locus have been demonstrated to prevent glycophosphatidylinositol (GPI) anchor synthesis and consequentially result in loss of GPI-anchored proteins from the cell's extracellular surface. The successful exploitation of this mutant phenotype in animal studies has triggered interest in the development of an analogous in vitro PIG-A mutation screening assay. This article describes the development of a robust assay design using metabolically active human cells. The assay includes viability and cell membrane integrity assessment and conforms to the future ideas of the 21st-century toxicology testing.

摘要

诱变剂可能是致癌物,传统上,它们是通过沙门氏菌“艾姆斯”反向突变试验在体外进行鉴定的。然而,原核生物的DNA包装、复制和修复系统在机制上与我们不可避免要保护的人类的这些系统有很大不同。因此,多年来一直使用能够检测真核生物诱变剂以及断裂剂和非整倍体剂的哺乳动物细胞系遗传毒性试验。这些主要基于啮齿动物的系统明显缺乏特异性,部分原因是它们的p53基因处于突变状态,这促使人们利用动物研究来解决数据冲突。最近,已证明PIG-A基因座的沉默突变会阻止糖基磷脂酰肌醇(GPI)锚的合成,从而导致GPI锚定蛋白从细胞外表面丢失。在动物研究中对这种突变表型的成功利用引发了人们对开发类似的体外PIG-A突变筛选试验的兴趣。本文描述了一种使用代谢活跃的人类细胞的稳健试验设计的开发。该试验包括活力和细胞膜完整性评估,并符合21世纪毒理学测试的未来理念。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/cd85/5907909/822e45324694/gew05901.jpg

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