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6/2010
vol. 6
 
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Basic research
Effect of repeated ischaemic preconditioning on TLR4 and proinflammatory cytokines TNF-α and IL-1β in myocardial ischaemia-reperfusion injury in a rat model

Ma Yu
,
Ni Wen
,
Zhu Wenzhong
,
Xiong Yuanchang
,
Deng Xiaoming
,
Luo Yongjin

Arch Med Sci 2010; 6, 6: 843-847
Online publish date: 2010/12/29
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- Effect of repeated.pdf  [0.09 MB]
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Introduction

Ischaemic heart disease is characterized by reduced blood supply to the cardiac muscle and is the primary cause of death associated with myocardial infarction usually occurring as a result of damage induced by cardiac ischaemia-reperfusion (I/R). Ischaemic preconditioning (IPC) is a phenomenon by which cyclic episodes of brief I/R protect the myocardium against subsequent lethal ischaemic injury. It is known to significantly reduce the infarct size, arrhythmia, and post-ischaemic contractile dysfunction [1, 2]. Ischaemic pre­conditioning (IPC) is a potent cellular protective mechanism that is initiated by brief periods of sublethal ischaemic stress. First identified by Murry et al., it has been concluded that the heart adapts within minutes to become resistant against ischaemia-induced injury.

The cellular mechanisms underlying the protection initiated by myocardial IPC have been scrutinized intensively, given the potential to identify novel targets for treating ischaemic heart disease. Work has focused on identifying the triggers, mediators, and end effectors of IPC. Numerous signal transduction pathways have been demonstrated to be mediators affording protection by IPC. Previous studies have demonstrated that phosphatidylinositol 3-kinase (PI3K) and its effector protein kinase B (Akt) are implicated in cell survival and that acute PI3K/Akt activation underlies the infarct size (IS)-limiting effect of ischaemic preconditioning (IP) in the rat heart [3-7]. A recent studies indicated that toll-like receptors (TLRs) are involved in the IP process [8, 9].

TLRs represent the first line of host defence against microbial infection and play a pivotal role in both innate and adaptive immunity. TLRs recognize invading pathogens through molecular pattern recognition, transduce signals via distinct intracellular pathways involving a unique set of adaptor proteins and kinases, and ultimately lead to the activation of transcription factors and inflammatory responses. Among 10 TLRs identified in humans, at least two exist in the heart, i.e., TLR2 and TLR4. In addition to the critical role of these in mediating cardiac dysfunction in septic conditions, emerging evidence suggests that the TLRs can also recognize endogenous ligands and may play an important role in modulating cardiomyocyte survival and in ischaemic myocardial injury [9].

The role of TLR4 in ischaemic preconditioning is still unclear; we do not know the change of the expression of TLR4 in the process. In this study we used ischaemic preconditioning models to observe the change of TLR4 expression and the level of proinflammatory cytokines TNF- and IL-1. Therefore, the purpose of this study was to determine the effect of TLR4 and proinflammatory cytokines TNF- and IL-1b that is involved in ischaemic preconditioning.

Material and methods

Myocardial I/R model and IP model protocol

Eighteen male Sprague-Dawley (SD) rats were randomly separated into sham (sham group), ischaemic reperfusion (IR group) and ischaemic preconditioning (IP group) groups (6/group). The I/R model and the surgical protocol were similar to methods described previously [10-12]. Rats were anaesthetized with urethane anaesthesia (5 ml/kg intraperitoneally). Atropine (0.05 mg s.c.) was administered to reduce airway secretions. Animals were orally intubated and connected to a mouse mini-ventilator. Core body temperature was maintained at 37°C with a heating pad and monitored with a rectal thermometer.

A median sternotomy was performed, and the left anterior descending coronary artery (LAD) was visualized and completely ligated for 30 min in I/R mice by tightening an 8-0 silk suture after passing it over a length of PE-10 tubing beneath the LAD at points 1-2 mm inferior to the left auricle. The 8-0 suture was similarly placed in the sham group but without LAD occlusion. The PE-10 tubing was ligated with the LAD to achieve easier ligature release and better reperfusion. Ischaemia was confirmed visually by the appearance of pale and bulging myocardium in the area at risk (AAR). The ligature was removed, and reperfusion was visually confirmed after 30 min of LAD occlusion. IPC was introduced by three cycles of 5 min ischaemia, followed by 5 min reperfusion, and repeated four times.

Measurement of serum TNF- and IL-1b level

Serum TNF- and IL-1b protein levels were measured by ELISA. Protein was extracted from the heart by pulverization of frozen tissue followed by extraction with lysis buffer containing protease inhibitors. Total protein was determined using a BCA Protein Assay kit (Pierce, Rockford, Illinois).

Western blot analysis

Tissue samples from the different groups were dissected. Tissues were homogenized in 500 ml of 25 mM Tris-HCl (pH 7.4) containing 1% Triton X-100, 0.1% sodium dodecyl sulfate (SDS), 2 mM EDTA, and 1% protease inhibitor cocktail (Sigma) and centrifuged at 14,0000 γ for 30 min at 4°C. The supernatants were used for Western blot analysis, with specific antibodies detecting TLR4 (Gen Script). Enhanced chemiluminescent (ECL) substrate was from Pierce (Rockford, IL, USA). The polyvinylidene difluoride (PVDF) membrane was from Schleicher and Schuell Co. (Hahnestrasse, Dassel, Germany). According to standard protocols, the blots were probed with primary antibodies, and horseradish peroxidase-conjugated secondary antibodies were used to reveal the specific protein bands with ECL detection reagents. The intensities of the protein bands were quantified by densitometry.

RT-PCR analysis

RNA was extracted from fresh rat tissues from the ischaemic area using Trizol (Gibco), according to the manufacturer’s instructions. RT-PCR analysis specific for TLR4 (Forward: 5’-GGACTCTGCCCTGCCACCATTTA-3’, Reverse: 5’-CTTGTGC CCTGTGAGGTCGTTGA-3’, anticipated size of PCR products 2800 bp) and -actin (Forward: 5'-GTCAGAAGGACTCCTACGTG-3', Reverse: 5'-TAGGAGCCA GGGCAGTAATC-3, anticipated size of PCR products 825 bp) was then performed using the RT-PCR kit (Takara Biotechnology) according to the manufacturer’s instructions.

Determination of myocardial infarct size

At the end of the perfusion protocols, the coronary artery was re-occluded and 4 ml of 0.1% Evans blue dye was injected into the aorta to delineate the area at risk. Stained hearts were frozen, sliced, and incubated at 37°C in 1% triphenyltetrazolium chloride to delineate infarcted tissue. Slices were then fixed and quantified. Infarct size was expressed as a percentage of the area at risk. The area at risk was calculated as a percentage of the total ventricular area.

Statistical analysis

Statistical analysis was done using SPSS 10.0. Parametric data were expressed as mean ± standard deviation (SD). Comparisons of parameters among the 3 groups were made with one-way ANOVA, followed by the Newman-Keuls test. Comparisons of parameters between 2 groups were made by unpaired Student's t test. A P value less than 0.05 was considered statistically significant.

Results

Serum level of TNF- and IL-1b

There were significant (P < 0.01) differences observed in the levels of TNF- and IL-1b between the I/R group and the sham group (Table I), and the levels decreased significantly (P < 0.01) in the IP group compared with the I/R group. The results showed that ischaemic preconditioning (IPC) protects the myocardium against lethal ischaemic injury induced by inflammatory factors TNF- and IL-1b.

RT-PCR analysis

The results (Figure 1) showed that the expression of TLR4 mRNA in the I/R group increased significantly (p < 0.01) compared with the sham group, but in the IP group the expression of TLR4 mRNA decreased significantly (p < 0.01) compared with the I/R group. The results indicated that ischaemic preconditioning inhibits the expression of TLR4 mRNA.

Western blot analysis

We found that the expression of TLR4 protein increased significantly (P < 0.01) in the I/R group compared with the sham group (Figure 2). There was no significant (P > 0.05) difference in the expression of b-actin in the 3 groups. When TLR4 protein levels were normalized with the expression of b-actin protein, the ratio was increased significantly (P < 0.01) in the I/R group compared with the sham group, whereas in the IP group the expression of TLR4 protein decreased significantly (P < 0.01) compared with the I/R group (Figure 2). These results suggest that TLR4 is activated in I/R, but ischaemic preconditioning inhibits the process.

Determination of myocardial infarct size

I/R increased the myocardial infarct size. Infarct size in the I/R group was greatly increased compared to the sham group (P < 0.01). As shown in Figure 3, the infarct size in the I/R group is 0.481 ±0.089; in the IP group (0.31 ±0.029) there was a significant decrease of myocardial infarct size versus the I/R group (P < 0.05).

Discussion

In our study, we found that the TLR4 protein level and mRNA level increased in the I/R process; at the same time TNF- and IL-1b level increased too. As we know, the expression of a constitutively active mutant of human Toll or Toll-like protein in the cell line activated the NF-kB pathway and the expression of NF-kB-mediated proinflammatory cytokines IL-1, TNF-, and others [13]. We also found that TLR4 and proinflammatory cytokines IL-1 and TNF- levels decreased in the IP process; these results indicated that the TLR4 signal and inflammation process are involved in the I/R and IP process. In addition, we found a significant decrease of myocardial infarct size in the IP group compared with the I/R group. So we can conclude that TLR4 and proinflammatory factors TNF- and IL-1b are involved in the IP process. To our knowledge, this is the first study showing that TLR4 and proinflammatory factors TNF- and IL-1b decreased in the IP process.

Frantz and colleagues first documented that there was enhanced TLR4 expression in remodelling murine myocardium remote from sites of ischaemic injury and in heart tissue from patients with idiopathic dilated cardiomyopathy [14]. In animal models of ischaemia-reperfusion injury or in hypoxic cardiomyocytes in vitro, the administration of a sublethal dose of lipopolysaccharide, which signals through TLR4, reduces subsequent myocardial infarction, improves cardiac functions, and attenuates cardiomyocyte apoptosis [15, 16]. By contrast, a systemic deficiency of TLR4 leads to attenuated myocardial inflammation, a smaller infarction size, better preserved ventricular function, and reduced ventricular remodelling after ischaemic injury [17, 18]. These recent studies demonstrate an emerging role for TLRs as a critical modulator in both cell survival and tissue injury in the heart. The precise molecular mechanisms responsible for the phenomenon are still unclear.

In summary, we found that the expression of TLR4 gene and protein decreased in the IP process. The preliminary data need to be well discussed and further studies carried out. It is possible that further studies of TLR4 will provide clues for better understanding of its function and may help uncover novel therapeutic strategies for regulating the I/R and IP process.

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