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Commentary Free access | 10.1172/JCI33706
Departments of Medicine and Cell Biology, Cardiovascular Research Center, and Cancer Center, Albert Einstein College of Medicine, New York, New York, USA.
Address correspondence to: Richard N. Kitsis, Albert Einstein College of Medicine, 1300 Morris Park Avenue, Bronx, New York 10461, USA. Phone: (718) 430-2609; Fax: (718) 430-8989; E-mail: kitsis@aecom.yu.edu.
Find articles by Whelan, R. in: JCI | PubMed | Google Scholar
Departments of Medicine and Cell Biology, Cardiovascular Research Center, and Cancer Center, Albert Einstein College of Medicine, New York, New York, USA.
Address correspondence to: Richard N. Kitsis, Albert Einstein College of Medicine, 1300 Morris Park Avenue, Bronx, New York 10461, USA. Phone: (718) 430-2609; Fax: (718) 430-8989; E-mail: kitsis@aecom.yu.edu.
Find articles by Mani, K. in: JCI | PubMed | Google Scholar
Departments of Medicine and Cell Biology, Cardiovascular Research Center, and Cancer Center, Albert Einstein College of Medicine, New York, New York, USA.
Address correspondence to: Richard N. Kitsis, Albert Einstein College of Medicine, 1300 Morris Park Avenue, Bronx, New York 10461, USA. Phone: (718) 430-2609; Fax: (718) 430-8989; E-mail: kitsis@aecom.yu.edu.
Find articles by Kitsis, R. in: JCI | PubMed | Google Scholar
Published October 1, 2007 - More info
Following myocardial infarction, nonischemic myocyte death results in infarct expansion, myocardial loss, and ventricular dysfunction. Here, we demonstrate that a specific proapoptotic gene, Bnip3, minimizes ventricular remodeling in the mouse, despite having no effect on early or late infarct size. We evaluated the effects of ablating Bnip3 on cardiomyocyte death, infarct size, and ventricular remodeling after surgical ischemia/reperfusion (IR) injury in mice. Immediately following IR, no significant differences were observed between Bnip3–/– and WT mice. However, at 2 days after IR, apoptosis was diminished in Bnip3–/– periinfarct and remote myocardium, and at 3 weeks after IR, Bnip3–/– mice exhibited preserved LV systolic performance, diminished LV dilation, and decreased ventricular sphericalization. These results suggest myocardial salvage by inhibition of apoptosis. Forced cardiac expression of Bnip3 increased cardiomyocyte apoptosis in unstressed mice, causing progressive LV dilation and diminished systolic function. Conditional Bnip3 overexpression prior to coronary ligation increased apoptosis and infarct size. These studies identify postischemic apoptosis by myocardial Bnip3 as a major determinant of ventricular remodeling in the infarcted heart, suggesting that Bnip3 may be an attractive therapeutic target.
Abhinav Diwan, Maike Krenz, Faisal M. Syed, Janaka Wansapura, Xiaoping Ren, Andrew G. Koesters, Hairong Li, Lorrie A. Kirshenbaum, Harvey S. Hahn, Jeffrey Robbins, W. Keith Jones, Gerald W. Dorn II
Much of the mortality following myocardial infarction results from remodeling of the heart after the acute ischemic event. Cardiomyocyte apoptosis has been thought to play a key role in this remodeling process. In this issue of the JCI, Diwan and colleagues present evidence that Bnip3, a proapoptotic Bcl2 family protein, mediates cardiac enlargement, reshaping, and dysfunction in mice without influencing infarct size (see the related article beginning on page 2825).
Thrombotic occlusion of an epicardial coronary artery triggers acute myocardial infarction. This cataclysmic event, which takes place approximately 1 million times per year in the US, sets into motion a spatially and temporally complex set of processes. In the region supplied by the occluded coronary artery (Figure 1), cardiomyocytes undergo massive cell death by apoptosis and necrosis (1). The sudden loss of a significant portion of myocardium leads to decreases in contractile function. These changes are compensated by increases in left-ventricular volume, which augment contractility in the noninfarcted myocardium via the Frank-Starling mechanism. A negative consequence of enhanced left-ventricular volume, however, is intensified wall stress. This is partially counteracted by scar formation in the infarct zone and cardiomyocyte hypertrophy in the noninfarcted myocardium. These mechanisms provide temporary compensation for the loss of myocardium. While most patients recover from acute myocardial infarction, those with larger infarcts often progress to chronic heart failure due to cardiac remodeling (2). This process involves both expansion of the infarct and changes in the geometry of the noninfarcted myocardium. The result is an enlarged, more spherical, and thin-walled left ventricle with poor contractile function. Drugs that attenuate postinfarct remodeling improve cardiac function and reduce mortality (2). The mechanisms underlying cardiac remodeling are incompletely understood, but inflammation (3), extracellular matrix remodeling (3), and cardiomyocyte hypertrophy (4) and apoptosis (5) have been implicated.
Postinfarct myocardial remodeling. Thrombotic occlusion of a coronary artery precipitates myocyte death in the ischemic zone creating a myocardial infarct (white area). The abrupt loss of functioning myocardium decreases contractile function. Acute compensation is provided by increases in left-ventricular volume (arrows) that augment function (the Frank-Starling mechanism) and neurohumoral factors that increase contractility in the noninfarcted myocardium. Augmented wall stress, a deleterious effect of increased left-ventricular volume, is reduced by myocyte hypertrophy in the noninfarcted myocardium (double-headed arrows). In addition, scar formation in the infarct limits expansion, preventing further increases in wall stress (not shown). In some patients, ventricular function is preserved. Other patients, especially those with larger infarcts, experience cardiac remodeling. In this process, the left ventricle undergoes dilation (dashed arrows), wall thinning, and a change in shape from ovoid to spherical, causing reduced contractile function and chronic heart failure. Strategies that inhibit postinfarct remodeling preserve left-ventricular geometry and function and prevent heart failure.
Apoptosis accounts for a significant portion of the large burst of cell death during acute myocardial infarction. Whole animal studies in which myocardial infarction was induced by ischemia/reperfusion (occlusion of a coronary artery followed by resumption of blood flow) have shown that genetic or pharmacologic inhibition of cardiomyocyte apoptosis decreases infarct size with concomitant preservation of cardiac function (6, 7). These studies indicate a causal role for cardiomyocyte apoptosis in the pathogenesis of infarction. In contrast to the infarct, lower levels of cardiomyocyte apoptosis are present in the noninfarcted myocardium in the weeks to months following infarction (5) and may play a role in remodeling and progression to heart failure (8).
Apoptosis is mediated by two pathways, one involving cell surface receptors and the other the mitochondria and endoplasmic reticulum (9). During apoptosis, the mitochondria are stimulated to release apoptogens, including cytochrome c, that activate downstream caspases and bring about the demise of the cell. The transmission of death signals to the mitochondria involves Bcl2 homology domain 3–only (BH3-only) proteins, a proapoptotic subclass of the Bcl2 family (10). BH3-only proteins are activated through transcriptional and posttranslational mechanisms and translocate to the outer mitochondrial membrane. Interactions between BH3-only proteins and multidomain Bcl2 proteins trigger the release of apoptogens, thereby causing apoptosis (11, 12).
Bcl2 and nineteen-kilodalton interacting protein–3 (Bnip3) is an atypical BH3-only protein because its BH3 domain possesses limited homology and, in contrast to typical BH3-only proteins, this domain is not required for cell death (13, 14). Bnip3 is present at low levels in several tissues, but its expression is markedly induced by hypoxia in a hypoxia-inducible factor–1α–dependent manner (15). In healthy cells, Bnip3 is loosely associated with mitochondria (16). In response to certain apoptotic signals, however, it inserts via a transmembrane domain into the outer mitochondrial membrane and triggers cell death. Whether this cell death occurs through apoptotic or nonapoptotic means remains controversial (17–21).
In this issue of the JCI, Diwan et al. inactivated Bnip3 in the mouse and gained insights into the role of apoptosis in cardiac remodeling (22). Loss of other BH3-only proteins has been shown to limit infarct size (23). Surprisingly, Diwan et al. found no difference in infarct size in wild-type and Bnip3-null mice subjected to ischemia/reperfusion. In contrast, Bnip3 ablation decreased apoptosis in the noninfarcted myocardium in the days following infarction. Moreover, the remodeling that takes place in the weeks following infarction was markedly attenuated in Bnip3-knockout mice as compared with wild-type mice. Increases in left-ventricular end-diastolic volume and sphericity were greater in wild-type mice than Bnip3-knockout mice. While systolic function decreased acutely in both groups following infarction, it continued to deteriorate in wild-type mice while stabilizing in Bnip3-knockout mice. These data indicate that Bnip3 mediates both cardiomyocyte death in the noninfarcted myocardium and cardiac remodeling.
How is it that Bnip3 is involved in cell death in the noninfarcted myocardium but not in the infarct itself? The authors posit that this may be attributable to differences in Bnip3 levels in these two zones. Bnip3 is expressed at low basal levels and induced by hypoxia in a variety of cell types, including cardiomyocytes (15, 24). While Bnip3 is sufficient to kill cardiomyocytes (18), there appears to be inadequate time for Bnip3 expression to increase in a developing infarction. On the other hand, one would predict robust induction of Bnip3 expression in the noninfarcted and severely hypoxic myocardium. To address these issues, it will be necessary to assess the temporal and spatial localization of hypoxia, Bnip3, and cell death in the postinfarct heart.
Diwan et al. (22) attributed improvement in postinfarct remodeling to inhibition of cardiomyocyte apoptosis in the noninfarcted myocardium. Postinfarct remodeling involves a complex interplay among multiple hematopoietic and resident cardiac cell types (3). The use of a generalized Bnip3 knockout in this study raises the question as to which cell type(s) mediate remodeling. Although Diwan et al. showed that the number and distribution of hematopoietic cells under basal conditions were unaffected by Bnip3 inactivation, these cells were not analyzed following recruitment into the milieu of the infarcting heart. As one example, macrophages in an infarct stimulate fibroblast proliferation and matrix remodeling and, after exerting their effects, undergo apoptosis (3). Since Bnip3 expression is induced by hypoxia in macrophages (25), it is possible that apoptosis of these cells in the healing infarct zone is impaired in Bnip3-knockout mice. Abnormal macrophage persistence could account for a thicker scar in the infarcts of Bnip3-knockout mice, as observed by Diwan et al., and resultant reductions in wall stress and ventricular dilation. If this hypothesis is correct, this sequence of events represents an additional mechanism — one that originates within the infarct zone rather than the noninfarcted myocardium — by which Bnip3 absence would ameliorate postinfarct remodeling. These effects of Bnip3 in the infarct zone may complement those described by Diwan et al. in the noninfarcted myocardium.
Limitation of infarct size and inhibition of remodeling are currently the cornerstones of therapy for myocardial infarction (2). Coronary reperfusion reduces infarct size, resulting in preservation of functional myocardium and thereby limiting the primary stimulus for remodeling. Postinfarct remodeling is inhibited using pharmacological (e.g., angiotensin I–converting enzyme [ACE] inhibitors) or mechanical unloading therapies in patients with significant systolic dysfunction. Despite optimal therapy, however, substantial numbers of patients progress to chronic heart failure following myocardial infarction. For this reason, there is a need for additional pharmacological strategies directed specifically against critical mediators of remodeling.
Bnip3 appears to be one such critical mediator of remodeling and possesses some attractive biological characteristics as a drug target. First, its site of action within the central death machinery may provide a target for specific inhibition of cell death. Second, its low basal levels in most tissues may minimize the possibility of untoward effects in nontarget organs. Third, the fact that Bnip3 is induced in response to hypoxia suggests that there is a temporal window, prior to significant Bnip3 accumulation and cell death, during which treatment could be beneficially instituted. Despite these characteristics, significant logistical hurdles exist in designing a practical pharmacological approach to inhibit this intracellular protein.
We thank Nikolaos G. Frangogiannis, Baylor College of Medicine, for helpful discussions. R.N. Kitsis is supported by NIH grants R01HL60665, R01HL61550, and R01HL80607, and the Dr. Gerald and Myra Dorros Chair in Cardiovascular Disease of the Albert Einstein College of Medicine. R.S. Whelan is supported by NIH grant T32AG23475.
Address correspondence to: Richard N. Kitsis, Albert Einstein College of Medicine, 1300 Morris Park Avenue, Bronx, New York 10461, USA. Phone: (718) 430-2609; Fax: (718) 430-8989; E-mail: kitsis@aecom.yu.edu.
Nonstandard abbreviations used: BH3, Bcl2 homology domain 3; Bnip3, Bcl2 and nineteen-kilodalton interacting protein–3.
Conflict of interest: The authors have declared that no conflict of interest exists.
Reference information: J. Clin. Invest.117:2751–2753 (2007). doi:10.1172/JCI33706.
See the related article at Inhibition of ischemic cardiomyocyte apoptosis through targeted ablation of Bnip3 restrains postinfarction remodeling in mice.