HSC70 is a chaperone for wild-type and mutant cardiac myosin binding protein C
Amelia A. Glazier, … , Adam S. Helms, Sharlene M. Day
Amelia A. Glazier, … , Adam S. Helms, Sharlene M. Day
Published June 7, 2018
Citation Information: JCI Insight. 2018;3(11):e99319. https://doi.org/10.1172/jci.insight.99319.
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Research Article Cardiology Muscle biology

HSC70 is a chaperone for wild-type and mutant cardiac myosin binding protein C

Abstract

Cardiac myosin binding protein C (MYBPC3) is the most commonly mutated gene associated with hypertrophic cardiomyopathy (HCM). Haploinsufficiency of full-length MYBPC3 and disruption of proteostasis have both been proposed as central to HCM disease pathogenesis. Discriminating the relative contributions of these 2 mechanisms requires fundamental knowledge of how turnover of WT and mutant MYBPC3 proteins is regulated. We expressed several disease-causing mutations in MYBPC3 in primary neonatal rat ventricular cardiomyocytes. In contrast to WT MYBPC3, mutant proteins showed reduced expression and failed to localize to the sarcomere. In an unbiased coimmunoprecipitation/mass spectrometry screen, we identified HSP70-family chaperones as interactors of both WT and mutant MYBPC3. Heat shock cognate 70 kDa (HSC70) was the most abundant chaperone interactor. Knockdown of HSC70 significantly slowed degradation of both WT and mutant MYBPC3, while pharmacologic activation of HSC70 and HSP70 accelerated degradation. HSC70 was expressed in discrete striations in the sarcomere. Expression of mutant MYBPC3 did not affect HSC70 localization, nor did it induce a protein folding stress response or ubiquitin proteasome dysfunction. Together these data suggest that WT and mutant MYBPC3 proteins are clients for HSC70, and that the HSC70 chaperone system plays a major role in regulating MYBPC3 protein turnover.

Authors

Amelia A. Glazier, Neha Hafeez, Dattatreya Mellacheruvu, Venkatesha Basrur, Alexey I. Nesvizhskii, Lap Man Lee, Hao Shao, Vi Tang, Jaime M. Yob, Jason E. Gestwicki, Adam S. Helms, Sharlene M. Day

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Figure 2

Interactions between MYBPC3 and molecular chaperones.

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Interactions between MYBPC3 and molecular chaperones. (A) Western blot s...
(A) Western blot showing co-IP of HSC70 and HSP70 with FLAG-tagged WT and mutant MYBPC3. Shorter MYBPC3 truncated proteins show loss of this interaction. (B) Summary of WT MYBPC3–interacting proteins manually categorized by function. All interactors were detected in both co-IP–MS experiments and showed a calculated fold change (FC-A) in spectral counts 2 or higher over nontransduced myocytes in at least one independent experiment. Interactors within dark boxes showed an FC-A of 2 or higher over background in both experiments. (C) Venn diagrams showing overlap of interacting proteins (left, all interactors; right, protein quality control interactors) identified in immunoprecipitates for WT, Ile154Leufs*5, and Trp1098* MYBPC3. MYBPC3 mutants show loss of interaction with protein quality control–related proteins. (DF) Normalized spectral counts for a subset of MYBPC3-interacting proteins from 2 independent co-IP–MS experiments. Adjusted spectral counts were normalized to abundance of FLAG-MYBPC3 bait protein. (D) HSC70 and HSP70 were more abundant in FLAG-Trp1098* samples, but less abundant in FLAG-Ile154Leufs*5 samples compared with FLAG-WT, while small heat shock proteins (E) showed loss of interaction with both mutants. (F) MYBPC3 mutants also showed reduced association with known binding partners myosin heavy chains α and β.