心脏原位巨噬细胞在小鼠心肌梗死后心脏修复中的作用  

作　　者：贾代乐 张景洪 陈圻炘 胡凯 孙爱军 葛均波 JIA Daile;ZHANG Jinghong;CHEN Qixin;HU Kai;SUN Aijun;GE Junbo(Department of Cardiology,Zhongshan Hospital,Fudan University,Shanghai Institute of Cardiovascular Diseases,State Key Laboratory of Cardiology,National Clinical Research Center for Interventional Medicine,Shanghai Clinical Research Center for Interventional Medicine,Shanghai 200032,China)

机构地区：[1]复旦大学附属中山医院心内科,上海市心血管病研究所,心脏病全国重点实验室,国家放射与治疗临床医学研究中心,上海市放射与治疗(介入治疗)临床医学研究中心,上海200032

出　　处：《中国临床医学》2024年第4期603-611,共9页Chinese Journal of Clinical Medicine

基　　金：国家自然科学基金(82100274);上海市青年科技英才扬帆计划(21YF1405900)。

摘　　要：目的探讨心脏原位巨噬细胞在小鼠心肌梗死后心脏修复中的作用及其机制。方法将巨噬细胞特异性Cre工具鼠(Cx3cr1CreER–YFP小鼠)与双重转基因小鼠(R26tdTomato/DTR小鼠)进行杂交,获得心脏原位巨噬细胞特异性红色荧光标记小鼠。选择60只Cx3cr1CreER–YFP:R26Td/DTR杂交小鼠,随机分为4组:假手术组(Sham组)、白喉毒素+假手术组(DT+Sham组)、心肌梗死模型组(MI组)和白喉毒素+心肌梗死模型组(DT+MI组),每组15只小鼠。MI组和DT+MI组采用结扎冠状动脉左前降支法进行心肌梗死造模,DT+MI组小鼠使用白喉毒素(diphtheria toxin,DT)诱导心脏组织中原位巨噬细胞的缺失,构建心脏原位巨噬细胞敲除模型。小鼠心肌梗死造模第5天,对小鼠心脏组织切片进行苏木精和伊红(H-E)染色,观察炎症浸润情况以及心肌梗死面积;造模第14天,采用超声心动图测定小鼠心功能相关指标,并检测炎性细胞因子mRNA表达水平。结果与MI组相比,DT+MI组小鼠心脏原位巨噬细胞明显减少[(53.75±4.62)vs(6.37±1.25),P<0.05]。心肌梗死造模14 d,与MI组相比,DT+MI组小鼠左心室舒张末期内径[(5.11±0.22)mm vs(5.92±0.26)mm,P<0.05]和收缩末期内径[(4.77±0.17)mm vs(5.38±0.16)mm,P<0.05]显著增大,而射血分数显著降低[(27.76±1.20)%vs(17.61±0.94)%,P<0.05];此外,DT+MI组小鼠心脏炎性细胞因子表达水平上升,炎症细胞浸润增加,心肌梗死面积明显增大。DT+MI组小鼠NF-κB/p-P65的蛋白表达水平显著高于MI组[(0.28±0.14)vs(1.09±0.12),P<0.05]。结论心脏原位巨噬细胞在心肌梗死后通过减轻炎症细胞浸润和心肌梗死面积,在心肌梗死后心脏组织修复中发挥重要作用。Objective To explore the role and mechanism of cardiac resident macrophages in heart repair after myocardial infarction in mice. Methods Macrophage-specific Cre tool mice(CX3CR1~(CreER-YFP) mice) with doubly transgenic mice(R26~(tdTomato/DTR) mice) were hybridized to obtain cardiac resident macrophage-specific red fluorescent labels in mice. Sixty Cx3cr1~(CreER-YFP):R26~(Td/DTR) hybrid mice were randomly divided into 4 groups: Sham group, DT+Sham group, MI group, and DT+MI group, with 15 mice in each group. MI group and DT+MI group underwent myocardial infarction modeling by ligating the left anterior descending coronary artery. The DT+MI group mice were induced to deplete resident macrophages in the heart tissue using diphtheria toxin(DT) to establish a cardiac resident macrophage knockout model. On the 5th day after myocardial infarction modeling, heart tissue slices of mice were stained with H-E to observe inflammation infiltration and myocardial infarct size were calculated;on the 14th day of modeling, echocardiography was used to measure cardiac function-related parameters in mice, and mRNA expression levels of inflammatory cytokines were detected. Results Compared with the MI group, the DT+MI group mice showed a significant reduction in cardiac resident macrophages([53.75±4.62] vs [6.37±1.25], P<0.05). On the 14th day after myocardial infarction modeling, compared with the MI group, the DT+MI group mice had significantly increased left ventricular end-diastolic diameter([5.11±0.22] mm vs [5.92±0.26] mm, P<0.05) and left ventricular end-systolic diameter([4.77±0.17] mm vs [5.38±0.16] mm, P<0.05), while the ejection fraction significantly decreased([27.76±1.20]% vs [17.61±0.94]%, P<0.05);in addition, the DT+MI group mice showed increased expression levels of inflammatory cytokines, increased inflammatory cell infiltration, and significantly larger myocardial infarct size. The protein expression levels of NF-κB/p-P65 in DT+MI group mice were significantly higher than those in the MI group([0.28±0.14]

关 键 词：心脏原位巨噬细胞 心肌梗死 心脏修复 

分 类 号：R735.7[医药卫生—肿瘤]