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On studying protein phosphorylation patterns using bottom-up LC-MS/ MS: the case of human alpha-casein

机译:使用自下而上的LC-MS / MS研究蛋白质磷酸化模式:以人α-酪蛋白为例

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Most proteomics studies involving mapping post-translational modifications, such as the phosphorylation of serine and threonine, are performed today using the 'bottom-up' approach. This approach involves enzymatic cleavage of proteins, most often by trypsin, with subsequent nano-LC-MS/MS. The occupancy rates of phosphosites in proteins may differ by orders of magnitude, and thus the occupancy rate must be reported for each occupied phosphosite. To highlight potential pitfalls in quantifying the occupancy rates, alpha_(s1)-casein from human milk was selected as a model molecule representing moderately phosphorylated proteins. For this purpose, human milk from one Caucasian woman in the eighth month of lactation was used. The phosphorylation level of caseins is believed to have major implications for the formation of micelles that are involved in delivering valuable calcium phosphate and other minerals to the newborn. Human alpha_(s1)-casein has been reported to be much less phosphorylated than ruminant caseins, which may indicate a different function of caseins in humans. Revealing the phosphorylation pattern in human casein can thus shed light on its function. The current study found that the sequence region between the residues Ser70 and Ser76 in human alpha_(s1)-casein is in fact phosphorylated, contrary to previous knowledge. The site of the most abundant phosphorylation is Ser75, in agreement with the known action of the mammary gland casein kinase. There is evidence for the second phosphorylation in that region, possibly at Ser73. Earlier reported positions of phosphorylations at Ser18 and Ser26 are also confirmed, but not the dominance of Ser18 phosphorylation. The occupancy rates at Ser18, Ser26 and Ser75 are estimated to be (7 + 2), (20 + 6) and (27 + 9)%, respectively. Owing to differences in the ionization efficiency between phosphorylated and unphosphorylated peptides a 30% error margin is added to the occupancy rates. The highlighted pitfalls of the bottom-up strategy include the sensitivity of enzymes to proximal acidic and phosphorylated residues and the presence of multiple isoforms, including unexpected ones, of the tryptic peptides. The utility of the earlier introduced PhosTS_hunter and ModifiComb approaches for evading the latter pitfall is demonstrated.
机译:如今,大多数蛋白质组学研究都涉及“翻译后修饰”的定位,例如丝氨酸和苏氨酸的磷酸化,是使用“自下而上”的方法进行的。这种方法涉及酶的蛋白质切割,通常是通过胰蛋白酶,随后是纳米LC-MS / MS。蛋白质中磷酸位的占用率可能相差一个数量级,因此必须报告每个占用的磷酸位的占用率。为了突出量化占用率的潜在陷阱,从人乳中选择α_(s1)-酪蛋白作为代表中等磷酸化蛋白的模型分子。为此,使用了哺乳期第八个月的一名白人妇女的母乳。酪蛋白的磷酸化水平被认为对胶束的形成有重要影响,胶束的形成涉及向新生儿传递有价值的磷酸钙和其他矿物质。与反刍动物酪蛋白相比,人类α_(s1)-酪蛋白的磷酸化程度要低得多,这可能表明酪蛋白在人类中的功能有所不同。因此,揭示人酪蛋白中的磷酸化模式可以阐明其功能。当前的研究发现,与先前的知识相反,人α_(s1)-酪蛋白中残基Ser70和Ser76之间的序列区域实际上已被磷酸化。与乳腺酪蛋白激酶的已知作用一致,最丰富的磷酸化位点是Ser75。有证据表明该区域可能在Ser73处发生了第二次磷酸化。还证实了先前报道的Ser18和Ser26磷酸化的位置,但没有证实Ser18磷酸化的优势。 Ser18,Ser26和Ser75的占用率分别估计为(7 + 2)%,(20 + 6)和(27 + 9)%。由于磷酸化和未磷酸化的肽之间的电离效率不同,因此在占用率上增加了30%的误差范围。自下而上策略的突出缺陷包括酶对近端酸性和磷酸化残基的敏感性以及胰蛋白酶肽的多种同工型的存在,包括意外的。演示了较早引入的PhosTS_hunter和ModifiComb方法规避后者陷阱的实用性。

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