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基因敲除的白色念珠菌菌株中可选择标记URA3的表达改变使毒力研究的解释变得复杂。

Altered expression of selectable marker URA3 in gene-disrupted Candida albicans strains complicates interpretation of virulence studies.

作者信息

Lay J, Henry L K, Clifford J, Koltin Y, Bulawa C E, Becker J M

机构信息

Microbiology Department, University of Tennessee, Knoxville, Tennessee 37919, USA.

出版信息

Infect Immun. 1998 Nov;66(11):5301-6. doi: 10.1128/IAI.66.11.5301-5306.1998.

Abstract

The ura-blaster technique for the disruption of Candida albicans genes has been employed in a number of studies to identify possible genes encoding virulence factors of this fungal pathogen. In this study, the URA3-encoded orotidine 5'-monophosphate (OMP) decarboxylase enzyme activities of C. albicans strains with ura-blaster-mediated genetic disruptions were measured. All strains harboring genetic lesions via the ura-blaster construct showed reduced OMP decarboxylase activities compared to that of the wild type when assayed. The activity levels in different gene disruptions varied, suggesting a positional effect on the level of gene expression. Because the URA3 gene of C. albicans has previously been identified as a virulence factor for this microorganism, our results suggest that decreased virulence observed in strains constructed with the ura-blaster cassette cannot accurately be attributed, in all cases, to the targeted genetic disruption. Although revised methods for validating a URA3-disrupted gene as a target for antifungal drug development could be devised, it is clearly desirable to replace URA3 with a different selectable marker that does not influence virulence.

摘要

在多项研究中采用了ura - 爆破技术来破坏白色念珠菌基因,以鉴定可能编码这种真菌病原体毒力因子的基因。在本研究中,对经ura - 爆破介导的基因破坏的白色念珠菌菌株的URA3编码的乳清苷5'-单磷酸(OMP)脱羧酶活性进行了测定。当进行测定时,所有通过ura - 爆破构建体携带遗传损伤的菌株与野生型相比,OMP脱羧酶活性均降低。不同基因破坏中的活性水平有所不同,表明对基因表达水平存在位置效应。由于白色念珠菌的URA3基因先前已被确定为该微生物的毒力因子,我们的结果表明,在所有情况下,用ura - 爆破盒构建的菌株中观察到的毒力降低不能准确地归因于靶向基因破坏。尽管可以设计出用于验证URA3破坏基因作为抗真菌药物开发靶点的修订方法,但显然需要用不影响毒力的不同选择标记取代URA3。

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