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The complete sequence and structural analysis of human apolipoprotein B-100: relationship between apoB-100 and apoB-48 forms.

机译:人载脂蛋白B-100的完整序列和结构分析:apoB-100和apoB-48形式之间的关系。

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摘要

We have isolated and sequenced overlapping cDNA clones covering the entire sequence of human apolipoprotein B-100 (apoB-100). DNA sequence analysis and determination of the mRNA transcription initiation site by S1 nuclease mapping showed that the apoB mRNA consists of 14,112 nucleotides including the 5' and 3' untranslated regions which are 128 and 301 nucleotides respectively. The DNA-derived protein sequence shows that apoB-100 is 513,000 daltons and contains 4560 amino acids including a 24-amino-acid-long signal peptide. The mol. wt of apoB-100 implies that there is one apoB molecule per LDL particle. Computer analysis of the predicted secondary structure of the protein showed that some of the potential alpha helical and beta sheet structures are amphipathic, whereas others have non-amphipathic neutral to apolar character. These latter regions may contribute to the formation of the lipid-binding domains of apoB-100. The protein contains 25 cysteines and 20 potential N-glycosylation sites. The majority of cysteines are distributed in the amino terminal portion of the protein. Four of the potential glycosylation sites are in predicted beta turn structures and may represent true glycosylation positions. ApoB lacks the tandem repeats which are characteristic of other apolipoproteins. The mean hydrophobicity the mean value of H1 and helical hydrophobic moment the mean value of microH profiles of apoB showed the presence of several potential helical regions with strong polar character and high hydrophobic moment. The region with the highest hydrophobic moment, between amino acid residues 3352 and 3369, contains five closely spaced, positively charged residues, and has sequence homology to the LDL receptor binding site of apoE. This region is flanked by three neighbouring regions with positively charged amino acids and high hydrophobic moment that are located between residues 3174 and 3681. One or more of these closely spaced apoB sequences may be involved in the formation of the LDL receptor-binding domain of apoB-100. Blotting analysis of intestinal RNA and hybridization of the blots with carboxy apoB cDNA probes produced a single 15-kb hybridization band whereas hybridization with amino terminal probes produced two hybridization bands of 15 and 8 kb. Our data indicate that both forms of apoB mRNA contain common sequences which extend from the amino terminal of apoB-100 to the vicinity of nucleotide residue 6300. These two messages may have resulted from differential splicing of the same primary apoB mRNA transcript.
机译:我们已经分离并测序了覆盖人载脂蛋白B-100(apoB-100)整个序列的重叠cDNA克隆。 DNA序列分析和通过S1核酸酶作图确定mRNA转录起始位点表明apoB mRNA由14,112个核苷酸组成,包括5'和3'非翻译区,分别为128和301个核苷酸。 DNA衍生的蛋白质序列显示apoB-100为513,000道尔顿,并包含4560个氨基酸,其中包括一个24个氨基酸长的信号肽。摩尔。 apoB-100的重量意味着每个LDL颗粒有一个apoB分子。对该蛋白质预测的二级结构的计算机分析表明,某些潜在的α螺旋和β折叠结构是两亲的,而另一些具有非两亲的中性至非极性特性。这些后面的区域可能有助于apoB-100的脂质结合域的形成。该蛋白质包含25个半胱氨酸和20个潜在的N-糖基化位点。大多数半胱氨酸分布在蛋白质的氨基末端部分。潜在的糖基化位点中的四个位于预测的β转角结构中,可能代表真正的糖基化位置。 ApoB缺乏其他载脂蛋白的串联重复序列。平均疏水性H1的平均值和螺旋疏水矩apoB的microH谱图的平均值表明存在几个具有强极性和高疏水矩的潜在螺旋区域。氨基酸残基3352和3369之间的疏水力矩最高的区域包含五个紧密间隔的带正电荷的残基,并且与apoE的LDL受体结合位点具有序列同源性。该区域的两侧是三个三个带正电荷氨基酸且疏水性高的相邻区域,位于残基3174和3681之间。这些紧密间隔的apoB序列中的一个或多个可能与apoB的LDL受体结合域的形成有关-100。肠道RNA的印迹分析和与羧基载脂蛋白B cDNA探针杂交的印迹产生了一条15kb的杂交带,而与氨基末端探针的杂交则产生了15和8kb的两条杂交带。我们的数据表明,两种形式的apoB mRNA均包含从apoB-100的氨基末端延伸至核苷酸残基6300附近的共有序列。这两种消息可能是由于相同的主要apoB mRNA转录物的差异剪接所致。

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