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猪蛔虫ABA-1多蛋白阵列中序列不同的单元具有相似的脂肪酸和视黄醇结合特性,但结合位点环境不同。

Sequence-divergent units of the ABA-1 polyprotein array of the nematode Ascaris suum have similar fatty-acid- and retinol-binding properties but different binding-site environments.

作者信息

Moore J, McDermott L, Price N C, Kelly S M, Cooper A, Kennedy M W

机构信息

Division of Infection and Immunity, Institute of Biomedical and Life Sciences, Joseph Black Building, University of Glasgow, Glasgow G12 8QQ, Scotland, UK.

出版信息

Biochem J. 1999 May 15;340 ( Pt 1)(Pt 1):337-43.

Abstract

Polyproteins comprise long polypeptides that are post-translationally cleaved into proteins of different function, or tandemly repetitive polypeptides which are processed into multiple versions of proteins which are presumed to have the same function. In the latter case the individual units of the polyprotein can differ substantially in sequence. Identity of function between the different units therefore cannot be assumed. Here we have examined the ABA-1 polyprotein allergen of the parasitic nematode Ascaris suum and found it to contain units which show a 50% difference in amino acid sequence. The parasite therefore produces at least two radically different forms of the allergen encoded within the polyprotein array. In fluorescence-based ligand-binding assays, recombinant polypeptides representing the two forms (designated ABA-1A1 and ABA-1B1) showed similar binding affinities for a range of fluorescent active-site probes [retinol, dansylundecanoic acid, dansyl-DL-alpha-amino-octanoic acid, cis-parinaric acid (cPnA)] and for the non-specific hydrophobic surface probe 8-anilinonaphthalene-1-sulphonic acid. However, the molecular environments in the active sites are markedly different, as indicated by disparate fluorescence emission peaks and intensities of bound probes. CD showed that the proteins have similar secondary structures but differ in susceptibility to chemical denaturation/unfolding by guanidinium chloride. Both retain a single conserved tryptophan residue in a characteristic non-polar environment, as revealed by extreme fluorescence blue shift. Thus the gross differences in sequence of the two proteins are not reflected in their ligand-binding specificities but in their binding-site environments.

摘要

多聚蛋白由长多肽组成,这些长多肽在翻译后被切割成具有不同功能的蛋白质,或者由串联重复多肽组成,这些多肽被加工成多种版本的蛋白质,推测具有相同的功能。在后一种情况下,多聚蛋白的各个单元在序列上可能有很大差异。因此,不能假定不同单元之间的功能相同。在这里,我们研究了寄生线虫猪蛔虫的ABA-1多聚蛋白过敏原,发现它包含氨基酸序列差异达50%的单元。因此,该寄生虫产生了至少两种在多聚蛋白阵列中编码的、截然不同的过敏原形式。在基于荧光的配体结合试验中,代表这两种形式的重组多肽(命名为ABA-1A1和ABA-1B1)对一系列荧光活性位点探针[视黄醇、丹磺酰十一烷酸、丹磺酰-DL-α-氨基辛酸、顺式十八碳四烯酸(cPnA)]以及非特异性疏水表面探针8-苯胺基萘-1-磺酸显示出相似的结合亲和力。然而,结合探针的荧光发射峰和强度不同,表明活性位点的分子环境明显不同。圆二色性显示这两种蛋白质具有相似的二级结构,但对氯化胍引起的化学变性/解折叠的敏感性不同。通过极端的荧光蓝移揭示,两者在特征性非极性环境中都保留了一个保守的色氨酸残基。因此,这两种蛋白质序列上的总体差异并未反映在它们的配体结合特异性上,而是反映在它们的结合位点环境中。

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