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The LCB2 gene of Saccharomyces and the related LCB1 gene encode subunits of serine palmitoyltransferase, the initial enzyme in sphingolipid synthesis.

机译:酿酒酵母的LCB2基因和相关的LCB1基因编码丝氨酸棕榈酰转移酶的亚基,该酶是鞘脂合成中的初始酶。

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摘要

The first and committed step in synthesis of the ceramide moiety of sphingolipids is catalyzed by serine palmitoyltransferase (EC 2.3.1.50), which condenses palmitoyl-CoA and serine to form 3-ketosphinganine. This step is thought to be tightly regulated to control the synthesis of sphingolipids, but data supporting this hypothesis are lacking mainly because the enzyme has resisted purification and consequent characterization. Rather than attempting to purify the enzyme from normal cells, we have taken a different tack and opted to try and overproduce the enzyme to facilitate its purification. Here we demonstrate that overproduction in Saccharomyces cerevisiae requires expression of LCB1, a previously isolated yeast gene, and LCB2, the isolation and characterization of which we describe. Several lines of evidence argue that both genes encode subunits of the enzyme; however, biochemical evidence will be needed to substantiate this hypothesis. Although overproduction was modest, 2- to 4-fold, it should now be possible to devise improved overproduction vectors for yeast or other host organisms.
机译:鞘脂的神经酰胺部分合成的第一步也是最重要的步骤是丝氨酸棕榈酰转移酶(EC 2.3.1.50)催化,该酶使棕榈酰-CoA和丝氨酸缩合形成3-ketosphinganine。该步骤被认为是严格调节的,以控制鞘脂的合成,但是缺少支持该假设的数据,主要是因为该酶具有抗纯化作用和随后的特征。我们没有尝试从正常细胞中纯化该酶,而是采取了另一种方法,选择尝试过量生产该酶以促进其纯化。在这里,我们证明酿酒酵母中的过量生产需要表达LCB1(先前分离的酵母基因)和LCB2(我们描述其分离和表征)。有几条证据表明,这两个基因都编码该酶的亚基。但是,将需要生物化学证据来证实这一假设。尽管过量生产是2到4倍,但现在应该有可能为酵母或其他宿主生物设计改良的过量生产载体。

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