首页> 外文期刊>Eukaryotic cell >Glycosyl Phosphatidylinositol-Anchored Proteins in Chemosensory Signaling: Antisense Manipulation of Paramecium tetraurelia PIG-A Gene Expression
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Glycosyl Phosphatidylinositol-Anchored Proteins in Chemosensory Signaling: Antisense Manipulation of Paramecium tetraurelia PIG-A Gene Expression

机译:化学传感信号中的糖基磷脂酰肌醇锚定蛋白:草履虫Pure-Pure-PIG-A基因表达的反义操纵。

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Glycosyl phosphatidylinositol (GPI)-anchored proteins are peripheral membrane proteins tethered to the cell through a lipid anchor. GPI-anchored proteins serve many functions in cellular physiology and cell signaling. The PIG-A gene codes for one of the enzymes of a complex that catalyzes the first step in anchor synthesis, and we have cloned the Paramecium tetraurelia pPIG-A gene using homology PCR. To understand the function of pPIG-A and the significance of GPI-anchored proteins in Paramecium, we reduced the mRNA for pPIG-A in transformed cells using an expression vector that transcribed antisense mRNA. The amount of transcript is reduced to ~0.3% of the mRNA in control-transformed cells. Compared to control cells, cells transformed with the antisense pPIG-A vector show reduced synthesis of GPI anchor intermediates catalyzed in their endoplasmic reticula and a very few GPI-anchored proteins among the peripheral proteins that can be recovered from their surfaces. They also show specific defects in chemoresponse to glutamate and folate. Other cellular functions, such as growth and mating, seem to be normal.
机译:糖基磷脂酰肌醇(GPI)锚定的蛋白是通过脂质锚栓拴在细胞上的外周膜蛋白。 GPI锚定的蛋白质在细胞生理学和细胞信号传导中起着许多功能。 PIG-A 基因编码催化锚合成的第一步的复合物的一种酶,我们已经使用同源性克隆了草履虫pureaure pPIG-A 基因。 PCR。为了了解 pPIG-A 的功能以及草履虫中GPI锚定蛋白的意义,我们在转化的植株中还原了 pPIG-A 的mRNA。细胞使用转录反义mRNA的表达载体。在对照转化细胞中,转录物的量减少到mRNA的〜0.3%左右。与对照细胞相比,用反义pPIG-A载体转化的细胞在其内质网中催化的GPI锚定中间体的合成减少,并且在外周蛋白中很少有GPI锚定的蛋白可以从其表面回收。它们还显示出对谷氨酸和叶酸的化学反应中的特定缺陷。其他细胞功能,例如生长和交配,似乎是正常的。

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