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两个大豆种子脂氧合酶突变体积累了脂氧合酶转录本的降低水平。

Two soybean seed lipoxygenase nulls accumulate reduced levels of lipoxygenase transcripts.

机构信息

Biochemistry Department, University of Missouri, 65212, Columbia, MO, U.S.A..

出版信息

Plant Mol Biol. 1986 Jan;7(1):11-23. doi: 10.1007/BF00020127.

Abstract

Soybean (Glycine max L. [Merrill]) seed lipoxygenase cDNA clones were recovered from two cDNA libraries: a size-selected library in pBR322 and an expression library in pUC8. The pUC8 library was made with total poly(A)(+) embryo RNA and was screened with antiserum to lipoxygenase-1, one of 3 seed lipoxygenase isozymes. Three lipoxygenase antigen-producing clones were identified: two with identical cDNA inserts of 977 nucleotides representing an open-reading frame and a third truncated clone bearing a 3' end common to the longer clones. A long clone, pAL-134, was chosen for further study and was used to screen the size-selected cDNA library from which sixteen clones were identified. They fall into two homology classes represented by pLX-10 (ca. 1360 bp) and pLX-65 (2047 bp).The lipoxygenase expression clone pAL-134 hybridized much more strongly to pLX-65 than to pLX-10. pAL-134 and pLX-65 share 89% nucleotide homology and 75% deduced amino acid homology along their common sequence. Their deduced amino acid sequences each show 80% homology to sequences determined for isolated peptides of the lipoxygenase-1 isozyme.pAL-134 hybridizes poorly with a 3.8 kb RNA from LOX-1 null (lx1) embryos while pLX-65 hybridizes more strongly, but still to a lesser extent than its hybridization to standard embryo RNA or to RNA from embryos lacking lipoxygenase-2 (lx2) or lipoxygenase-3 (lx3) protein.The lx3 null lacks almost all embryo 3.8 kb RNA homologous to pLX-10. This hybridization pattern suggests that pLX-10 encodes LOX-3. Thus, the lx1 and lx3 genotypes accumulate little, if any, mRNA for the lipoxygenase-1 and lipoxygenase-3 isozymes, respectively.

摘要

从两个 cDNA 文库中回收了大豆(Glycine max L. [Merrill])种子脂氧合酶 cDNA 克隆:一个在 pBR322 中进行大小选择的文库和一个在 pUC8 中进行表达的文库。pUC8 文库是用总 poly(A)(+)胚胎 RNA 构建的,并用抗脂氧合酶-1 的抗血清筛选,脂氧合酶-1 是 3 种种子脂氧合酶同工酶之一。鉴定出了 3 个产生脂氧合酶抗原的克隆:两个具有相同的 977 个核苷酸的 cDNA 插入物,代表一个开放阅读框,第三个截短的克隆带有与较长克隆共有的 3'末端。选择长克隆 pAL-134 进行进一步研究,并用于筛选大小选择的 cDNA 文库,从中鉴定出 16 个克隆。它们分为两个同源类,由 pLX-10(约 1360 bp)和 pLX-65(2047 bp)表示。脂氧合酶表达克隆 pAL-134 与 pLX-65 的杂交比与 pLX-10 的杂交强得多。pAL-134 和 pLX-65 在其共同序列上具有 89%的核苷酸同源性和 75%的推导氨基酸同源性。它们的推导氨基酸序列彼此都与分离的脂氧合酶-1 同工酶肽的序列显示出 80%的同源性。pAL-134 与 LOX-1 缺失(lx1)胚胎的 3.8 kb RNA 杂交不良,而 pLX-65 杂交更强,但仍不如其与标准胚胎 RNA 或缺乏脂氧合酶-2(lx2)或脂氧合酶-3(lx3)蛋白的胚胎 RNA 的杂交。lx3 缺失几乎没有与 pLX-10 同源的所有胚胎 3.8 kb RNA。这种杂交模式表明 pLX-10 编码 LOX-3。因此,lx1 和 lx3 基因型分别积累很少,如果有的话,脂氧合酶-1 和脂氧合酶-3 同工酶的 mRNA。

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