2018
DOI: 10.1016/j.yjmcc.2018.07.247
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Temperature-sensitive sarcomeric protein post-translational modifications revealed by top-down proteomics

Abstract: Despite advancements in symptom management for heart failure (HF), this devastating clinical syndrome remains the leading cause of death in the developed world. Studies using animal models have greatly advanced our understanding of the molecular mechanisms underlying HF; however, differences in cardiac physiology and the manifestation of HF between animals, particularly rodents, and humans necessitates the direct interrogation of human heart tissue samples. Nevertheless, an ever-present concern when examining … Show more

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Cited by 20 publications
(23 citation statements)
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References 71 publications
(83 reference statements)
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“…RNA and protein degradation is an obvious way to detect a 'bad' sample. A particularly sensitive test is the level of protein phosphorylation, since, counter-intuitively, if tissue is not frozen soon enough or thaws out later, the level of TnI phosphorylation increases (Cai et al 2018).…”
Section: Discussionmentioning
confidence: 99%
“…RNA and protein degradation is an obvious way to detect a 'bad' sample. A particularly sensitive test is the level of protein phosphorylation, since, counter-intuitively, if tissue is not frozen soon enough or thaws out later, the level of TnI phosphorylation increases (Cai et al 2018).…”
Section: Discussionmentioning
confidence: 99%
“…LV myocardium from nonfailing hearts from brain-dead donors with no history of heart diseases but unsuitable for heart transplant were used as control tissues in this study (Ctrl, n = 16). The donor hearts LV tissues were obtained either from the University of Wisconsin Organ and Tissue Donation ( 67 69 ) or from the Sydney Heart Bank. Interventricular septal myocardium from patients with obstructive HCM undergoing septal myectomy surgery ( 30 ) for relief of symptoms was analyzed in this study (HCM, n = 16).…”
Section: Methodsmentioning
confidence: 99%
“…Sarcomeric proteins were extracted as previously reported, with minor modifications ( 67 ). To minimize artificial protein modifications and oxidation, tissue homogenization was performed at 4 °C.…”
Section: Methodsmentioning
confidence: 99%
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“…Prior reports by the Ge group have established N-terminal trimethylation of RLCV and phosphorylation of swine RLCV, but phosphorylation of human RLCV was unlocalized and observed at <10% stoichiometry. 58,59 The removal of N-terminal methionine and trimethylation was confirmed by tandem HCD fragmentation, and the site of phosphorylation was localized to S15, which is analogous to the site identified on swine RLCV (Figure 5B). On a last analytical note, phosproteoforms of cardiac troponin I (cTnI) 60 were not separated by RPLC but were at baseline by CZE (Figure 5C); proteoform quantitation by both techniques showed <10% coefficient of variation between them.…”
Section: Unique Proteoforms Are Reflective Of Tissue Central Functionmentioning
confidence: 56%