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秀丽隐杆线虫的P-糖蛋白基因家族。基因组和互补DNA序列的克隆与特性分析。

The P-glycoprotein gene family of Caenorhabditis elegans. Cloning and characterization of genomic and complementary DNA sequences.

作者信息

Lincke C R, The I, van Groenigen M, Borst P

机构信息

Netherlands Cancer Institute, Division of Molecular Biology, Amsterdam.

出版信息

J Mol Biol. 1992 Nov 20;228(2):701-11. doi: 10.1016/0022-2836(92)90855-e.

Abstract

P-glycoproteins, encoded by families of evolutionarily conserved genes, can confer a multidrug-resistant phenotype to mammalian tumor cells. To obtain more information on their functions in normal cells we have cloned genomic and complementary DNA sequences of four P-glycoprotein gene homologs of the genetically well-characterized nematode Caenorhabditis elegans, termed pgp-1, pgp-2, pgp-3 and pgp-4, respectively. The genes were physically mapped on chromosome IV (pgp-1), I (pgp-2) and X (pgp-3 and pgp-4). Phenotypic mutants corresponding to these loci have not yet been described. Two of the genes, pgp-1 and pgp-3, were analyzed in detail. They are predicted to encode ATP-binding membrane-spanning proteins of 1321 and 1254 amino acid residues, respectively, with the characteristic features shared by most P-glycoproteins described thus far. Intra-species divergence of P-glycoprotein genes is more pronounced in C. elegans than in mammals. Only 40% of the amino acids of pgp-1 and pgp-3 are identical, in contrast to 77% identity between human MDR1 and MDR3. pgp-1 consists of 14 exons, pgp-3 of 13. The two genes share only one intron position, whereas they share four (pgp-1) and five (pgp-3) intron positions with mammalian P-glycoprotein genes. pgp-1, pgp-2, and pgp-3 are transcribed into low abundance mRNAs in wild-type nematodes. pgp-1 and pgp-3 mRNAs have the trans-spliced leader SL1 at their 5' ends. Arsenite, emetine and actinomycin D drugs did not increase the steady state levels of pgp mRNA, unlike in some mammalian cell types. Heat shock disturbed trans as well as cis-splicing of pgp-1 and led to the accumulation of partially processed pgp-1 RNA. Thus, in C. elegans these genes are not induced in the context of a general stress response, as has been proposed for mammalian P-glycoprotein genes in certain tissues.

摘要

由进化保守基因家族编码的P-糖蛋白可赋予哺乳动物肿瘤细胞多药耐药表型。为了获取更多关于它们在正常细胞中功能的信息,我们克隆了遗传特征明确的线虫秀丽隐杆线虫的四个P-糖蛋白基因同源物的基因组和互补DNA序列,分别命名为pgp-1、pgp-2、pgp-3和pgp-4。这些基因在物理上定位于第四条染色体(pgp-1)、第一条染色体(pgp-2)和X染色体(pgp-3和pgp-4)上。尚未描述与这些位点相对应的表型突变体。对其中两个基因pgp-1和pgp-3进行了详细分析。预计它们分别编码由1321和1254个氨基酸残基组成的ATP结合跨膜蛋白,具有迄今为止描述的大多数P-糖蛋白共有的特征。秀丽隐杆线虫中P-糖蛋白基因的种内差异比哺乳动物中更为明显。pgp-1和pgp-3只有40%的氨基酸相同,相比之下,人类MDR1和MDR3之间的同一性为77%。pgp-1由14个外显子组成,pgp-3由13个外显子组成。这两个基因仅共享一个内含子位置,而它们与哺乳动物P-糖蛋白基因分别共享四个(pgp-1)和五个(pgp-3)内含子位置。pgp-1、pgp-2和pgp-3在野生型线虫中转录为低丰度mRNA。pgp-1和pgp-3 mRNA在其5'端具有反式剪接前导序列SL1。与某些哺乳动物细胞类型不同,亚砷酸盐、吐根碱和放线菌素D药物不会增加pgp mRNA的稳态水平。热休克干扰了pgp-1的反式和顺式剪接,并导致部分加工的pgp-1 RNA积累。因此,在秀丽隐杆线虫中,这些基因不像某些组织中哺乳动物P-糖蛋白基因那样在一般应激反应中被诱导。

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