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Epigenetic silencing of gene expression in Entamoeba histolytica.

机译:溶组织变形虫中基因表达的表观遗传沉默。

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Transcriptional silencing of an amebapore (ap-a) gene occurred in Entamoeba histolytica following the transfection of plasmids containing a DNA segment (473 bp) homologous to the 5' upstream region of the gene. This segment contains the promoter region of the ap-a gene, a T-rich stretch, followed by a truncated SINE1 (short interspersed element) that is transcribed from the opposite strand. The downstream silencing of the ap-a gene did not occur with plasmids containing the entire SINE1 sequence or lacking the entire SINE1 sequences including the T-rich stretch. Such plasmids promoted the overexpression of the ap-a gene. The transcription of the SINE element required both the T-rich stretch as well as sequences from the 5' end of SINE. RNA extracts from gene-silenced cultures showed small amounts of short (approximately 140 nt), single-stranded molecules with homology to SINE1 transcripts but no siRNA. Chromatin immunoprecipitation (ChIP) analysis of silenced G3 trophozoites with an antibody against methylated K4 of histone H3 revealed a demethylation of K4 at the domain of the ap-a gene indicating transcriptional inactivation. These results suggest the involvement of the SINE1 element in triggering the gene silencing and the role of histone modification in its epigenetic maintenance. The avirulent phenotype of the silenced trophozoites was demonstrated in various assays and the results suggest they may have a potential use for vaccination.
机译:在转染含有与该基因的5'上游区域同源的DNA片段(473 bp)的质粒后,在变形虫变形杆菌中发生了甲孔(ap-a)基因的转录沉默。该区段包含ap-a基因的启动子区域,富含T的延伸序列,后面是截短的SINE1(短散元素),其从相反的链转录而来。对于包含完整SINE1序列或缺少完整SINE1序列(包括富T序列)的质粒,ap-a基因的下游沉默没有发生。这样的质粒促进了ap-a基因的过表达。 SINE元件的转录既需要富T的延伸,也需要来自SINE 5'末端的序列。来自基因沉默培养物的RNA提取物显示出少量的短链(约140 nt)单链分子,与SINE1转录本具有同源性,但没有siRNA。用抗组蛋白H3甲基化K4的抗体对沉默的G3滋养体进行染色质免疫沉淀(ChIP)分析,发现ap-a基因域中K4脱甲基,表明转录失活。这些结果表明SINE1元素参与触发基因沉默和组蛋白修饰在其表观遗传维持中的作用。沉默的滋养体的无毒表型在各种试验中得到证实,结果表明它们可能具有潜在的疫苗接种用途。

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