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白色念珠菌中编码1,3-β-葡糖基转移酶的BGL2基因破坏后的表型。

Phenotype in Candida albicans of a disruption of the BGL2 gene encoding a 1,3-beta-glucosyltransferase.

作者信息

Sarthy Aparna V, McGonigal Thomas, Coen Michael, Frost David J, Meulbroek Jonathan A, Goldman Robert C

机构信息

Anti-infective Research Division, D47M/AP9A, 100 Abbott Park Road, Abbott Laboratories, Abbott Park, IL 60064-3500, USA.

出版信息

Microbiology (Reading). 1997 Feb;143 ( Pt 2):367-376. doi: 10.1099/00221287-143-2-367.

Abstract

The BGL2 gene encodes a unique 1,3-beta-glucosyltransferase (Bgl2p) present in the cell wall of Candida albicans and other fungi. Although believed to be involved in cell wall assembly, disruption of the gene in saccharomyces cerevisiae showed no apparent phenotype. We performed sequential disruptions of the BGL2 loci in a homozygous ura3 clinical isolate of C. albicans using the URA3 blaster method, in order to investigate the role of Bgl2p in this dimorphic, pathogenic fungus. Strain CACW-1 contained disruptions of both homologues of the BGL2 gene and lacked Bgl2p, as assessed by protein extraction, SDS-PAGE and Western blot analysis, and enzyme assay; however, residual non-Bgl2p transferase activity was detected. CACW-1 was attenuated in virulence for mice when compared to an isogenic parent strain, and fewer organisms were recovered from the kidneys of infected animals. Additional phenotypic changes included: (1) a dramatic increase in the sensitivity to the chitin synthesis inhibitor nikkomycin Z when CACW-1 cells were incubated at 37 or 42 degrees C; (2) an 8.7 +/- 1.6% slower growth rate at 37 degrees C for CACW-1 when compared to its isogenic parent; and (3) aggregation of CACW-1 cells during stationary phase and/or incubation of stationary phase cells in phosphate buffer. Characterization of SDS-extracted cell walls did not reveal any significant differences in the levels of 1,3-beta- or 1,6-beta-glucan. These data reveal that loss of Bgl2p does have a phenotype in C. albicans, and indicate that (1) loss of Bgl2p function renders cells more dependent on chitin for wall integrity, and attenuates virulence (probably due to subtle changes in wall structure), and (2) that additional 1,3-beta-glucosyltransferases are present in the C. albicans BGL2 disruptant.

摘要

BGL2基因编码一种独特的1,3-β-葡糖基转移酶(Bgl2p),该酶存在于白色念珠菌和其他真菌的细胞壁中。尽管人们认为它参与细胞壁组装,但在酿酒酵母中破坏该基因并未表现出明显的表型。我们使用URA3爆破法在白色念珠菌的纯合ura3临床分离株中对BGL2基因座进行了连续破坏,以研究Bgl2p在这种二态性致病真菌中的作用。通过蛋白质提取、SDS-PAGE、蛋白质印迹分析和酶活性测定评估,菌株CACW-1的BGL2基因的两个同源物均被破坏,且缺乏Bgl2p;然而,检测到了残留的非Bgl2p转移酶活性。与同基因亲本菌株相比,CACW-1对小鼠的毒力减弱,从感染动物的肾脏中回收的菌体数量更少。其他表型变化包括:(1)当CACW-1细胞在37或42℃孵育时,对几丁质合成抑制剂多氧霉素Z的敏感性显著增加;(2)与同基因亲本相比,CACW-1在37℃时的生长速率慢8.7±1.6%;(3)在稳定期CACW-1细胞聚集,和/或在磷酸盐缓冲液中孵育稳定期细胞时聚集。对SDS提取的细胞壁的表征未发现1,3-β-葡聚糖或1,6-β-葡聚糖水平有任何显著差异。这些数据表明,Bgl2p的缺失在白色念珠菌中确实具有表型,并表明:(1)Bgl2p功能的丧失使细胞在细胞壁完整性方面更依赖几丁质,并减弱毒力(可能是由于细胞壁结构的细微变化),(2)白色念珠菌BGL2破坏株中存在其他1,3-β-葡糖基转移酶。

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