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Phosphorylation of B14.5a subunit from bovine heart complex I identified by titanium dioxide selective enrichment and shotgun proteomics

机译:二氧化钛选择性富集和shot弹枪蛋白质组学鉴定牛心复合体B14.5a亚基的磷酸化。

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摘要

Shotgun proteomics was used to study the steady phosphorylation state of NADH:ubiquinone oxidoreductase (complex I) subunits from bovine heart mitochondria. A total tryptic digestion of enzymatically active complex I was performed, and the resulting peptide mixture was subjected to phosphopeptide enrichment by the use of titanium dioxide (TiO2). The phosphopeptide-enriched fraction was separated and analyzed with nanoscale reverse-phase HPLC-ESI-MS/MS in single information-dependent acquisition. Hence two phosphorylated complex I subunits were detected: 42 kDa and B14.5a. Phosphorylation of 42-kDa subunit at Ser-59 has already been determined with fluorescent phosphoprotein-specific gel staining and mass spectrometry (Schilling, B., Aggeler, R., Schulenberg, B., Murray, J., Row, R. H., Capaldi, R. A., and Gibson, B. W. (2005) Mass spectrometric identification of novel phosphorylation site in subunit NDUFA10 of bovine mitochondrial complex I. FEBS Lett. 579, 2485-2490). In our work, this finding was confirmed using a non-gel-based approach. In addition, we report novel phosphorylation on B14.5a nuclear encoded subunit. We demonstrated evidence of the phosphorylation site at Ser-95 residue by collision-induced dissociation experiments on three different molecular ions of two tryptic phosphopeptides of B14.5a.
机译:弹枪蛋白质组学用于研究牛心脏线粒体中NADH:泛醌氧化还原酶(复合I)亚基的稳定磷酸化状态。进行酶活性复合物I的总胰蛋白酶消化,并使用二氧化钛(TiO2)对所得的肽混合物进行磷酸肽富集。分离富含磷酸肽的级分,并以纳米级反相HPLC-ESI-MS / MS进行单信息依赖采集。因此,检测到两个磷酸化的复合物I亚基:42kDa和B14.5a。已经通过荧光磷蛋白特异性凝胶染色和质谱法确定了Ser-59处42 kDa亚基的磷酸化(Schilling,B.,Aggeler,R.,Schulenberg,B.,Murray,J.,Row,RH,Capaldi ,RA,和Gibson,BW(2005)质谱鉴定牛线粒体复合体I的NDUFA10亚单位中的新磷酸化位点I. FEBS Lett。579,2485-2490)。在我们的工作中,使用非基于凝胶的方法证实了这一发现。此外,我们报告B14.5a核编码的亚基上的新型磷酸化。我们通过碰撞诱导的离解实验对B14.5a的两个胰蛋白酶磷酸肽的三个不同分子离子证明了Ser-95残基的磷酸化位点。

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