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Identification of post-translational modifications resulting from LHbeta polymorphisms by matrix-assisted laser desorption time-of-flight mass spectrometric analysis of pituitary LHbeta core fragment

机译:由LHBETA多态性通过基质辅助激光解吸飞行时间质谱分析垂直LHBETA核心片段的转移后修饰的鉴定

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摘要

Metabolism of the human chorionic gonadotrophin (hCG)- and LHbeta-subunits (hCGP, LHbeta) terminates with the urinary excretion of core fragment (hCGbetacf, LHbetacf) molecules that retain antigenic shape and constituent N-linked carbohydrate moieties. We have previously demonstrated the resolved mass spectra of hCGbetacf, from which the carbohydrate moieties present at two N-linked glycosylation sites were identified. LHbetacf was subjected to the same mass spectrometric analysis. As LHbeta shares 82% homology with hCGbeta but possesses only one glycosylation consensus site a simpler spectral fingerprint of LHbetacf glycoforms was expected. LHbetacf was reduced with dithiothreitol and analysed by matrix-assisted laser desorption/ionisation time-of-flight mass spectrometry. Glycoforms were predicted by subtracting the peptide mass from the m/z values of the observed peaks and then sequentially subtracting the masses of the monosaccharide residues of hCGbeta N-linked carbohydrates reported in the literature. The mass spectra of LHbetacf revealed a broad single peak ranging from m/z 8700 to 10 700. Following reduction, this peak was replaced by a set of partially resolved peaks between m/z 4130 and 5205 corresponding to glycosylated forms of the peptide LHbeta6-40. A peak at m/z 4252-2 corresponded to the non-glycosylated peptide LHbeta55-93. Remaining peaks indicated that the pooled sample comprised a wide set of glycoforms, contained LHbetacf with two N-linked carbohydrate moieties and indicated evidence of further glycosylation due to amino acid substitution in polymorphic variants. This is evidence that a single nucleotide polymorphism alters the post-translational modification of a protein and hence its structural phenotype.
机译:人绒毛膜促性腺激素(HCG)和LHBETA-亚基(HCGP,LHBETA)的代谢终止于核心片段(HCGBetacf,LHBetacf)分子的尿液排泄,其保留抗原形状和组分N-连接的碳水化合物部分。我们之前已经证明了HCGBetacf的已解析质谱,鉴定了两个N个连接糖基化位点的碳水化合物部分。对LHBetacf进行相同的质谱分析。由于LHBETA与HCGBETA股份,但只有一个糖基化共识位点,预计LHBETACF糖族的更简单的光谱指纹。用二硫噻钛糖醇降低了Lhbetacf,并通过基质辅助激光解吸/电离飞行时间质谱法分析。通过从观察到的峰的M / Z值中减去肽质量来预测糖型,然后依次减去文献中报道的HCGBeta N-连接碳水化合物的单糖残余物的质量。 Lhbetacf的质谱显示出从M / Z 8700至10 700的宽单峰。在还原后,将该峰被与糖基化形式的M / Z 4130和5205之间的一组部分分辨的峰取代,所述肽Lhbeta6- 40。 M / Z 4252-2的峰值对应于非糖基化肽LHBETA55-93。剩余的峰表明,汇集样品包括含有含有含有两种N链碳水化合物的Lhbetacf,并指出由于多态性变体中的氨基酸取代而进一步的糖基化的证据。这证明单个核苷酸多态性改变了蛋白质的翻译后修饰,从而改变了其结构表型。

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    ES Jacoby; AT Kicman; RK Iles;

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  • 年度 2003
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  • 正文语种 eng
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