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首页> 外文期刊>Medical mycology: official publication of the International Society for Human and Animal Mycology >The LAMMER kinase is involved in morphogenesis and response to cell wall- and DNA-damaging stresses in Candida albicans
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The LAMMER kinase is involved in morphogenesis and response to cell wall- and DNA-damaging stresses in Candida albicans

机译:Lammer激酶参与了形态发生和对Candida albicans中的细胞壁和DNA损伤应力的反应

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摘要

Dual specificity LAMMER kinase has been reported to be conserved across species ranging from yeasts to animals and has multiple functions. Candida albicans undergoes dimorphic switching between yeast cells and hyphal growth forms as its key virulence factors. Deletion of KNS1, which encodes for LAMMER kinase in C. albicans, led to pseudohyphal growth on YPD media and defects in filamentous growth both on spider and YPD solid media containing 10% serum. These cells exhibited expanded central wrinkled regions and specifically reduced peripheral filaments. Among the several stresses tested, the kns1 Delta strains showed sensitivity to cell-wall and DNA-replicative stress. Under fluorescent microscopy, an increase in chitin decomposition was observed near the bud necks and septa in kns1 Delta cells. When the expression levels of genes for cell wall integrity (CWI) and the DNA repair mechanism were tested, the kns1 double-deletion cells showed abnormal patterns compared to wild-type cells; The transcript levels of genes for glycosylphosphatidylinositol (GPI)-anchored proteins were increased upon calcofluor white (CFW) treatment. Under DNA replicative stress, the expression of MluI-cell cycle box binding factor (MBF)-targeted genes, which are expressed during the G1/S transition in the cell cycle, was not increased in the kns1 double-deletion cells. This strain showed increased adhesion to the surface of an agar plate and zebrafish embryo. These results demonstrate that Kns1 is involved in dimorphic transition, cell wall integrity, response to DNA replicative stress, and adherence to the host cell surface in C. albicans.
机译:据报道,双重特异性Lammer激酶在从酵母到动物的种类中保存,并且具有多种功能。念珠菌白醛人在酵母细胞和亚腿生长形式之间进行二态切换,作为其关键毒力因子。缺失KNS1,在C.醛糖盆中编码牙齿激酶,导致YPD培养基上的假小鼠生长,捕获含有10%血清的蜘蛛和YPD固体培养基中的丝状生长缺陷。这些细胞表现出膨胀的中央皱纹区域,并特别减少外周细丝。在测试的几种应力中,KNS1 DELTA菌株表明对细胞壁和DNA复制应力的敏感性。在荧光显微镜下,在KNS1δ细胞的芽颈和隔膜附近观察到甲壳素分解的增加。当测试细胞壁完整性(CWI)基因的表达水平和DNA修复机理时,与野生型电池相比,KNS1双缺失细胞显示出异常模式;在Copofluor白色(CFW)处理时增加了糖基磷脂酰磷脂肌醇(GPI)-Achered蛋白的基因的转录物水平。在DNA复制应激下,在Cells循环中的G1 / S转变期间表达的Mlui细胞周期箱结合因子(MBF)的表达在KNS1双缺失细胞中未增加。该菌株显示出对琼脂板和斑马鱼胚的表面增加的粘附性。这些结果表明,KNS1涉及二态转变,细胞壁完整性,对DNA复制应激的响应,以及在C.醛族人中粘附到宿主细胞表面。

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