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Single-Cell RNA Sequencing Reveals that the Switching of the Transcriptional Profiles of Cysteine-Related Genes Alters the Virulence of Entamoeba histolytica

机译:单细胞RNA测序表明,半胱氨酸相关基因的转录谱的切换改变了entamoeba组织olyolytica的毒力

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Entamoeba histolytica is an intestinal protozoan that causes human amoebic colitis and extraintestinal abscesses. Virulence variation is observed in the pathogenicity of E. histolytica trophozoites, but the detailed mechanism remains unclear. Here, a single trophozoite was cultured alone, and the progeny of the trophozoites of each generation were subjected to single-cell RNA sequencing (scRNA-seq) to study the transcriptional profiles of trophozoites. The scRNA-seq analysis indicated the importance of sulfur metabolism and the proteasome pathway in pathogenicity, whereas the isobaric tags for relative and absolute quantitation (iTRAQ) proteomic analysis did not identify the bulk trophozoites. The trophozoite improved the synthesis of cysteine under cysteine-deficient conditions but downregulated the expression of the intermediate subunit of the lectin of E. histolytica trophozoites and retained the expression of the heavy subunit of lectin, resulting in decreased amoebic phagocytosis and cytotoxicity. The variation in the transmembrane kinase gene family might be critical in regulating the proteasome pathway. Thus, the scRNA-seq technique provided an improved understanding of the biological characteristics and the mechanism of virulence variation of amoebic trophozoites. IMPORTANCE Studies on the trophozoite of Entamoeba histolytica suggested this organism could accumulate polyploid cells in its proliferative phase and differentiate its cell cycle from that of other eukaryotes. Therefore, a single-cell sequencing technique was used to study the switching of the RNA transcription profiles of single amoebic trophozoites. We separated individual trophozoites from axenic cultured trophozoites, CHO cell-incubated trophozoites, and in vivo trophozoites. We found important changes in the sulfur and cysteine metabolism in pathogenicity. The trophozoites strategically regulated the expression of the cysteine-rich protein-encoding genes under cysteine-deficient conditions, thereby decreasing amoebic phagocytosis and cytotoxicity. The single-cell sequencing technique shows evident advantages in comparison with the isobaric tags for relative and absolute quantitation (iTRAQ) proteomic technology (bulk trophozoite level) and reveals the regulation strategy of trophozoites in the absence of exogenous cysteine. This regulation strategy may be the mechanism of virulence variation of amoebic trophozoites.
机译:entamoeba histolytica是一种肠道原生动物,导致人类雄染结肠炎和外来脓肿。在E.组织晶粒滋养体的致病性中观察到毒力变异,但是详细机制仍不清楚。这里,单独培养单一的滋养体,对每种一代的滋养体的后代进行单细胞RNA测序(ScRNA-SEQ)以研究滋养体的转录谱。 SCRNA-SEQ分析表明硫代谢和致病性致病性的重要性,而相对和绝对定量(ITRAQ)蛋白质组学分析的表征标签没有识别散装滋养体。滋养体改善了半胱氨酸缺乏条件下半胱氨酸的合成,但下调了大素凝集素的中间亚基的表达,并保留了凝集素的重亚基的表达,导致氨基吞噬作用和细胞毒性降低。跨膜激酶基因家族的变异对于调节蛋白酶体途径可能是至关重要的。因此,SCRNA-SEQ技术提供了改善对生物特征的理解和Amoebic Trophocozoites的毒力变异机制。对entamoeba组织族晶体滋生的重要性研究表明这种有机体可以在其增殖阶段积累多倍体细胞,并将其细胞周期与其他真核生物的循环分化。因此,使用单细胞测序技术来研究单个氨基滋生蛋白的RNA转录谱的切换。我们将个体滋养体从腋生培养的滋养性,CHO细胞培养的滋养性和体内滋养色谱中分开。我们在致病性中发现了硫和半胱氨酸代谢的重要变化。滋养体策略性地调节富含半胱氨酸缺乏条件下的半胱氨酸富含蛋白质编码基因的表达,从而降低了氨基吞噬作用和细胞毒性。单细胞测序技术表现出与相对和绝对定量(ITRAQ)蛋白质组学技术(散装滋养色素水平)的同位素标签相比明显的优势,并揭示了在没有外源性半胱氨酸的情况下滋养化的调控策略。该调节策略可能是Amoebic滋养本质的毒力变异机制。

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