Cell-specific ablation of Hsp47 defines the collagen-producing cells in the injured heart
Hadi Khalil, Onur Kanisicak, Ronald J. Vagnozzi, Anne Katrine Johansen, Bryan D. Maliken, Vikram Prasad, Justin G. Boyer, Matthew J. Brody, Tobias Schips, Katja K. Kilian, Robert N. Correll, Kunito Kawasaki, Kazuhiro Nagata, Jeffery D. Molkentin
Hadi Khalil, Onur Kanisicak, Ronald J. Vagnozzi, Anne Katrine Johansen, Bryan D. Maliken, Vikram Prasad, Justin G. Boyer, Matthew J. Brody, Tobias Schips, Katja K. Kilian, Robert N. Correll, Kunito Kawasaki, Kazuhiro Nagata, Jeffery D. Molkentin
View: Text | PDF
Research Article Cardiology

Cell-specific ablation of Hsp47 defines the collagen-producing cells in the injured heart

Abstract

Collagen production in the adult heart is thought to be regulated by the fibroblast, although cardiomyocytes and endothelial cells also express multiple collagen mRNAs. Molecular chaperones are required for procollagen biosynthesis, including heat shock protein 47 (Hsp47). To determine the cell types critically involved in cardiac injury–induced fibrosis the Hsp47 gene was deleted in cardiomyocytes, endothelial cells, or myofibroblasts. Deletion of Hsp47 from cardiomyocytes during embryonic development or adult stages, or deletion from adult endothelial cells, did not affect cardiac fibrosis after pressure overload injury. However, myofibroblast-specific ablation of Hsp47 blocked fibrosis and deposition of collagens type I, III, and V following pressure overload as well as significantly reduced cardiac hypertrophy. Fibroblast-specific Hsp47-deleted mice showed lethality after myocardial infarction injury, with ineffective scar formation and ventricular wall rupture. Similarly, only myofibroblast-specific deletion of Hsp47 reduced fibrosis and disease in skeletal muscle in a mouse model of muscular dystrophy. Mechanistically, deletion of Hsp47 from myofibroblasts reduced mRNA expression of fibrillar collagens and attenuated their proliferation in the heart without affecting paracrine secretory activity of these cells. The results show that myofibroblasts are the primary mediators of tissue fibrosis and scar formation in the injured adult heart, which unexpectedly affects cardiomyocyte hypertrophy.

Authors

Hadi Khalil, Onur Kanisicak, Ronald J. Vagnozzi, Anne Katrine Johansen, Bryan D. Maliken, Vikram Prasad, Justin G. Boyer, Matthew J. Brody, Tobias Schips, Katja K. Kilian, Robert N. Correll, Kunito Kawasaki, Kazuhiro Nagata, Jeffery D. Molkentin

×

Figure 7

Hsp47 deletion in myofibroblasts reduces ECM-related gene expression and promotes an altered differentiated state.

Options: View larger image (or click on image) Download as PowerPoint
Hsp47 deletion in myofibroblasts reduces ECM-related gene expression an...
(A) Adult primary heart fibroblasts were isolated from Hsp47-loxP–targeted mice infected with Adβgal (WT) or AdCre (deleted samples). Seventy-two hours after infection cells were washed and incubated in 2% serum containing DMEM media with 20 μM ascorbic acid for 24 hours before RNA isolation. The data are real-time PCR results showing the expression levels of the indicated genes. n = 4 separate experiments. *P < 0.05 versus Adβgal WT. (B) Schematic representation of the Postn-MCM mouse line crossed with the Hsp47-loxP site–containing gene–targeted line and the Rosa26 reporter line (R26eGFP). (C) Experimental scheme with TAC stimulation and tamoxifen with injection and laden food. (D and E) Quantification of selected mRNAs in Hsp47-deleted EGFP+ myofibroblasts isolated from hearts of Hsp47fl/flPostn-MCM/+R26eGFP/+ allele containing mice, 4 weeks after TAC injury. n = 3, *P < 0.5. P values were calculated with Student’s t test. Data shown are the mean ± SEM.