Correlation between apoptosis and left ventricular remodeling in subacute phase of myocardial ischemia and reperfusion

Cardiomyocyte death by apoptosis during ischemia-reperfusion and myocardial infarction (MI) is associated with the progression of left ventricular (LV) dysfunction and remodeling [1‐3]. The progressive loss of cardiomyocytes after acute MI (AMI) and ischemia-reperfusion may play a key role in the pathogenesis of heart failure.

Apoptosis is triggered through two main pathways: (1) the intrinsic pathway involves mitochondria and cytoplasmic reticulum, and (2) the extrinsic pathway utilizes cell surface receptor. Cellular stresses such as infarction and ischemia-reperfusion induce apoptosis through the intrinsic pathway [4‐7]. These stimuli lead to the release of several factors into cytosol including cytochrome c, which activates the initiator caspase-9 via the apoptosome followed by the activation of effector caspases. The activation of downstream caspases leads to the cleavage of numerous structural and regulatory cellular proteins, thereby producing the apoptotic phenotype characterized by cell shrinkage, chromatin condensation, nucleus fragmentation, and externalization of phosphatidylserine (PS) on the outside of the cell membrane that serves as a signal for phagocytes. Annexin-V, a member of a phospholipid binding family of proteins, binds to PS-containing sites on the cell surface and has been suggested to be an early marker of apoptosis. Then, radiolabeled annexin-V has been used for the detection of apoptosis as a noninvasive imaging tool [8].

The process of myocardial tissue repair and healing after AMI is considered to consist of four phases based on the pathologic findings: cardiomyocyte death, acute inflammation, formation of granulation tissue, and scar formation [9]. After 2 weeks of MI, granulation tissue formation in the ischemic area is ongoing. The granulation tissue is still rich in inflammatory cells like lymphocytes and macrophages for helping to clear the cellular debris. At this point, the prolonged ^99mTc-annexin-V uptake by cardiomyocyte might correlate with a variety of tissue repair and healing.

Our previous studies showed that ^99mTc-annexin-V binding commenced at 0.5 h after ischemia-reperfusion in the mid-myocardium within the area at risk (AAR) and expanded to the subendocardial and subepicardial layers at 6 h after ischemia-reperfusion in rat models [10, 11]. The ^99mTc-annexin-V binding diminished gradually over 3 days and continued till 2 weeks after reperfusion. However, we could not assess the relation between ^99mTc-annexin-V uptake and LV remodeling, because we only had investigated five rats with 20 min of ischemia at 2 weeks after reperfusion.

Therefore, we investigated whether apoptosis or cell death demonstrated by ^99mTc-annexin-V uptake correlated with LV remodeling in rat models of myocardial ischemia-reperfusion at 2 weeks after reperfusion.

Significant ^99mTc-annexin-V uptake was (1) frequently documented in the AAR in 10 rats (66 % of all rats), especially in the case of a longer ischemia (100 % for 30 min of ischemia vs. 44 % for 20 min, P < 0.05) and (2) correlated with LV DI (mean value ± SD; 0.18 ± 0.06 vs. 0.06 ± 0.03, P = 0.0017) and LV WTR (mean value ± SD; 0.66 ± 0.10 vs. 1.08 ± 0.05, P < 0.0001), whereas it did not correlate with the ratio of AAR to the whole LV (mean value ± SD; 0.51 ± 0.04 vs. 0.41 ± 0.06, P = 0.1). Only two rats with 30 min of ischemia had ^99mTc-annexin-V uptake in both the AAR and normally perfused area adjacent to the AAR. LV DI and WTR were correlated with ^99mTc-annexin-V uptake ratio [correlate coefficient = 0.70 (P = 0.0036) and −0.81 (P = 0.0002), respectively] (Fig. 2). Representative cases were shown in Fig. 3.

In the rats with 20 and 30 min of ischemia, light microscopic examination of the HE slices from frozen specimens showed that necrotic myocardium was replaced by granulation tissues with inflammatory cells. Scattered TUNEL-positive cells were detected in the AAR in rats with AV uptake, whereas TUNEL-positive cells were minimally observed in rats without ^99mTc-annexin-V uptake. Representative HE and TUNEL staining was shown in Fig. 4.

The present study confirmed that ^99mTc-annexin-V uptake was observed at 2 weeks after LCA occlusion and reperfusion in rats with a dilated LV cavity and thinned wall using autoradiography. Since ^99mTc-annexin-V uptake might reflect ongoing cell death of cardiomyocytes, the detection of apoptosis can be used as a diagnostic tool for predicting loss of cardiomyocytes in the vulnerable myocardial areas during the postinfarction recovery period.

^99mTc-annexin-V uptake seems to depend on the severity of ischemia-reperfusion injury in the rat model. Previous investigations demonstrated that apoptosis was observed at AAR after short-time ischemia and that apoptosis was involved extensively in border zone after long-time ischemia [15]. In this study, the size ratio of AAR to whole LV was not different between LCA occlusion time, but ^99mTc-annexin-V uptake in the AAR was significantly more observed in 30 min in the LCA occlusion model. Our results agreed with the previous findings that myocardial apoptosis appeared in ischemia-reperfusion area and that apoptosis was useful to evaluate ischemia-reperfusion damage.

Loss of myocardium caused by apoptosis in the acute phase of MI contributed to progressive myocardial dysfunction in human clinical studies. Human clinical studies demonstrated that increased uptake of ^99mTc-annexin-V was present in the infarct area in patients with AMI after percutaneous coronary intervention [16, 17]. In these studies, timing of monitoring apoptosis was based on the acute phase of MI, because apoptosis of myocardium was observed most strongly in the acute phase after ischemic damage.

Then, how long has apoptosis been observed in rat model? Palojoki et al. [18] showed that cardiomyocyte apoptosis occurred continuously over an extended period of time in the viable border zones of infarct scars in a rat model of permanent ligation. TUNEL-positive cardiomyocytes were numerous at 1 day after LCA ligation in both the viable border zones and the central infarct areas (average value 4.39 and 1.44 %). At later time points, scattered TUNEL-positive cardiomyocytes were observed in both the border zones adjacent to infarct scars and the remote myocardium (average value 0.34 and 0.09 % at 4 weeks, 0.10 and 0.04 % at 12 weeks, respectively).

Cardiomyocyte apoptosis occurs in advanced heart failure after the acute phase of MI. Olivetti et al. [19] demonstrated the existence of cardiomyocyte apoptosis morphologically and biochemically in patients who underwent cardiac transplantation for intractable congestive heart failure. Abbate et al. [20] examined an apoptotic rate (AR), the ratio of the number of cardiomyocytes co-expressing positive TUNEL and caspase-3 on nucleated cells per field, in both the infarct and the remote area in patients dying ≥10 days after AMI. The higher AR in the infarct area correlated with relative LV cavity dilation strongly but AR in the remote area did not. Apoptotic rate at the site of the infarction was increased nearly fourfold in patients with symptomatic heart failure at the time of initial hospitalization for AMI or subsequently before death versus remaining patients (median value 26.2 vs. 6.4 %). Our results consisted with their findings in that the positive ^99mTc-AV uptake in the AAR correlated with LV cavity dilation and thinned wall. Interestingly, the two rats demonstrated significant uptake expanded over the border zone between ischemic and normally perfused area after ischemia and reperfusion. Although apoptotic cardiomyocytes in remote non-infarcted areas contribute to the LV remodeling in rodent models of permanent ligation [18, 21, 22], such an apoptotic process over border zones in subacute phase had not been reported. In this respect, further study would be warranted to determine the significance of ^99mTc-AV uptake in the normally perfused area.

^99mTc-annexin-V uptake in injured myocardium correlated with LV remodeling at 2 weeks after myocardial ischemia-reperfusion. Ischemia-driven apoptosis or cell death demonstrated by ^99mTc-annexin-V uptake in the subacute phase might be a possible marker of LV remodeling.