Identification and cloning of GCA1, a gene that encodes a cell surface glucoamylase from Candida albicans

白色念珠菌 生物 酵母 分子生物学 半乳糖 基因 打开阅读框 生物化学 白色体 基因组文库 同源(生物学) 肽序列 微生物学
作者
Joy Sturtevant,Freddie Dixon,E Wadsworth,Jean‐Paul Latgé,Xiao Zhao,Richard Calderone
出处
期刊:Medical Mycology [Oxford University Press]
卷期号:37 (5): 357-366 被引量:1
标识
DOI:10.1111/j.1365-280x.1999.00244.x
摘要

Adherence of yeast cells of Candida albicans to human oesophageal cells is greater when cells are grown in 500 m m D-galactose in comparison to d-glucose at the same concentration. Moreover, a 190 kDa mannoprotein (MP190) from a yeast cell wall preparation is highly expressed when cells are grown in the presence of galactose but less so in glucose. We now report on the identification of the MP190 and the isolation of its encoding gene. MP190 was purified, and three internal peptides were isolated and sequenced. Each of the three peptides showed significant homology (65–85%) with a glucoamylase (GAM1) from the yeast, Schwanniomyces occidentalis. In order to isolate the C. albicans homologue of GAM1 (GCA1), we probed a genomic library with a 0·9-kb internal fragment of the S. occidentalis GAM1 and isolated a 2·3-kb clone that corresponded to the 5′ region of the gene. Polymerase chain reaction (PCR) amplification was used to isolate the remainder of the open reading frame. GCA1 encodes a 946 amino acid protein containing three putative hydrophobic, membrane-spanning domains and 15 potential N-glycosylation sites. Both Gca1p and GAM1 are novel to the family of glycosyl hydrolases. Northern analysis indicated that GCA1 is transcribed to a greater extent in galactose than in sucrose or glucose. Also, using reverse transcriptase (RT)-PCR, we observed expression of GCA1 in a rat model of oral candidiasis, indicating that Gca1p is expressed during disease development.
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