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布氏锥虫S427cl1菌株在无菌条件下G1期到S期细胞周期进程的调控

Control of G1 to S cell cycle progression of Trypanosoma brucei S427cl1 organisms under axenic conditions.

作者信息

Morgan G A, Laufman H B, Otieno-Omondi F P, Black S J

机构信息

Department of Microbiology, Ohio State University, Columbus 43210-1292.

出版信息

Mol Biochem Parasitol. 1993 Feb;57(2):241-52. doi: 10.1016/0166-6851(93)90200-h.

Abstract

Trypanosoma brucei S427cl1 organisms made 6 divisions in modified minimal essential medium (BMEM) supplemented with fetal bovine serum (FBS)-low or high density lipoprotein (LDL, HDL) and fatty acid-free bovine serum albumin (FAF-BSA). Omission of lipoproteins or FAF-BSA from the medium caused the parasites to accumulate in G1 of the cell cycle and to lose the ability to replicate at 37 degrees C. Proteinase K-treated LDL or HDL, which did not have detectable apolipoprotein, supported the G1 to S cell cycle transition of T. brucei S427cl1 organisms in BMEM supplemented with FAF-BSA. Addition of C6:0, C7:0 or fatty C8:0 fatty acid (1 mol fatty acid mol-1 FAF-BSA in the incubation mixture) to serum-free medium supplemented with LDL or HDL and FAF-BSA prevented T. brucei S427cl1 organisms from progressing through G1 into S of the cell cycle. T. brucei S427cl1 organisms became stumpy-like forms during plateau phase growth under axenic conditions. Stumpy-like T. brucei S427cl1 organisms were mainly in G1 of the cell cycle, expressed raised levels of NAD diaphorase activity, were unable to replicate at 37 degrees C, but were able to differentiate to replicating procyclic organisms. Medium collected from plateau phase cultures of T. brucei S427cl1 did not support the G1 to S cell cycle transition of exponentially growing T. brucei organisms. The capacity of plateau phase medium to support G1 to S transition of T. brucei S427cl1 organisms was restored by addition of FAF-BSA and its capacity to support 4 cycles of replication of the parasites was restored by addition of FAF-BSA and LDL or HDL.

摘要

布氏锥虫S427cl1生物体在添加了胎牛血清(FBS)、低密度脂蛋白(LDL)或高密度脂蛋白(HDL)以及无脂肪酸牛血清白蛋白(FAF-BSA)的改良基本培养基(BMEM)中进行了6次分裂。培养基中缺少脂蛋白或FAF-BSA会导致寄生虫在细胞周期的G1期积累,并失去在37℃下复制的能力。经蛋白酶K处理的LDL或HDL(其中未检测到载脂蛋白),在添加了FAF-BSA的BMEM中支持布氏锥虫S427cl1生物体从G1期向S期的细胞周期转变。向添加了LDL或HDL以及FAF-BSA的无血清培养基中添加C6:0、C7:0或脂肪酸C8:0(孵育混合物中1摩尔脂肪酸/摩尔FAF-BSA)可阻止布氏锥虫S427cl1生物体从G1期进入细胞周期的S期。在无菌条件下的平台期生长过程中,布氏锥虫S427cl1生物体变成了类似粗短型的形态。类似粗短型的布氏锥虫S427cl1生物体主要处于细胞周期的G1期,表达升高的NAD黄递酶活性,无法在37℃下复制,但能够分化为可复制的前循环生物体。从布氏锥虫S427cl1的平台期培养物中收集的培养基不支持指数生长的布氏锥虫生物体从G1期向S期的细胞周期转变。通过添加FAF-BSA可恢复平台期培养基支持布氏锥虫S427cl1生物体从G1期向S期转变的能力,通过添加FAF-BSA以及LDL或HDL可恢复其支持寄生虫4个复制周期的能力。

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