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ω-3 二十二碳六烯酸由大鼠 Elovl5 和 Elovl2 差异伸长的分子基础。

Molecular basis for differential elongation of omega-3 docosapentaenoic acid by the rat Elovl5 and Elovl2.

机构信息

Rheumatology Unit, Royal Adelaide Hospital, SA, Australia.

出版信息

J Lipid Res. 2013 Oct;54(10):2851-7. doi: 10.1194/jlr.M041368. Epub 2013 Jul 21.

Abstract

Functional characterization of the rat elongases, Elovl5 and Elovl2, has identified that Elovl2 is crucial for omega-3 docosahexaenoic acid (DHA) (22:6n-3) synthesis. While the substrate specificities of the rat elongases had some overlap, only Elovl2 can convert the C22 omega-3 PUFA docosapentaenoic acid (DPA) (22:5n-3) to 24:5n-3, which is the penultimate precursor of DHA. In order to better understand the potential for these elongases to be involved in DHA synthesis, we have examined the molecular reasons for the differences between Elovl5 and Elovl2 in their ability to elongate DPA to 24:5n-3. We identified a region of heterogeneity between Elovl5 and Elovl2 spanning transmembrane domains 6 and 7. Using a yeast expression system, we examined a series of Elovl2/Elovl5 chimeras and point mutations to identify Elovl2 residues within this region which are responsible for DPA substrate specificity. The results indicate that the cysteine at position 217 in Elovl2 and a tryptophan at the equivalent position in Elovl5 explain their differing abilities to elongate DPA to 24:5n-3. Further studies confirmed that Elovl2 C217 is a critical residue for elongation of DPA at the level observed in the native protein. Understanding the ability of elongases to synthesize 24:5n-3 may provide a basis for using sequence data to predict their ability to ultimately support DHA synthesis.

摘要

大鼠延伸酶 Elovl5 和 Elovl2 的功能特征鉴定出 Elovl2 对于 ω-3 二十二碳六烯酸 (DHA) (22:6n-3) 的合成至关重要。虽然大鼠延伸酶的底物特异性有些重叠,但只有 Elovl2 可以将 C22 ω-3 多不饱和脂肪酸二十二碳五烯酸 (DPA) (22:5n-3) 转化为 24:5n-3,这是 DHA 的倒数第二个前体。为了更好地理解这些延伸酶在 DHA 合成中的潜在作用,我们研究了 Elovl5 和 Elovl2 在将 DPA 延伸为 24:5n-3 的能力上存在差异的分子原因。我们确定了 Elovl5 和 Elovl2 之间在跨膜域 6 和 7 之间存在异质性区域。使用酵母表达系统,我们研究了一系列 Elovl2/Elovl5 嵌合体和点突变,以鉴定该区域中 Elovl2 残基负责 DPA 底物特异性。结果表明,Elovl2 中的 217 位半胱氨酸和 Elovl5 中相同位置的色氨酸解释了它们将 DPA 延伸为 24:5n-3 的不同能力。进一步的研究证实,Elovl2 的 C217 是在天然蛋白中观察到的 DPA 延伸的关键残基。了解延伸酶合成 24:5n-3 的能力可能为使用序列数据预测它们最终支持 DHA 合成的能力提供基础。

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