Objective: To explore whether CD137-CD137L signaling mediated exocytosis of autophagosome within vascular smooth muscle cells (VSMCs) could influence the formation of atherosclerotic calcification. Methods: Fifteen 8-week-old male ApoE(-/-)(C57BL/6J-KO) mice fed with high fat diet for 5 weeks were randomly divided into three groups by using stochastic indicator method as follows: control group, n=5; agonist-CD137 group: agonist-CD137 antibody 200 μg/2 weeks for 4 weeks, ip, n=5; anti-CD137 group: 200 μg anti-CD137 antibody+ 200 μg agonist-CD137 antibody/2 weeks for 4 weeks, ip, n=5. Von Kossa staining was applied to observe the calcification of the thoracic aortic atherosclerotic plaque in each group. Immunohistochemistry was used to detect the expression of LC3 and Beclin1 which were the autophage markers of early-to-mid stage; Western blot was adopted to quantify protein level of microtubule-associated proteins 1 light chain 3B(LC3B) and mammalian ortholog of the yeast autophagy-related gene 6 (Beclin1). Transmission electron microscope (TME) was used to observe the formation of autophagosome in plaque. C57BL/6J mouse VSMCs were cultured by using tissue piece inoculation method. Groups of in vitro studies were the same as in vivo study: control group, agonist-CD137 group, anti-CD137 group, the agonist-CD137 groups was treated with agonist-CD137 antibody (10 μg/ml) and anti-CD137 group was treated with anti-CD137 antibody (10 μg/ml) for 30 minutes, followed by agonist-CD137 antibody (10 μg/ml). Von Kossa staining and osteogenesis phenotypic alkaline phosphatase (ALP) activity detection were adopted to observe calcification in VSMCs. Autophagosomes were separated from the supernatant of the agonist-CD137 group with density gradient centrifugation method. VSMCs were divided into two groups: positive group (containing complete medium with above autophagosomes to a final concentration 15 μg/ml) and negative group (only complete medium) after being pretreated with mixed inflammatory cytokines (IL-1β、IFN-γ and TNF-α, final concentration was 25 ng/ml respectively) for 24 hours and calcium deposition and osteogenesis phenotypic marker bone morphogenetic protein 2(BMP2) were then detected. Results: (1) Compared with the control group, activation of the CD137-CD137L signal significantly increased the formation of calcification area in thoracic aortic atherosclerotic plaque of ApoE(-/-) mice((1.82±0.15)×10(4) μm(2) vs. (0.34±0.08)×10(4) μm(2,) P<0.01), this effect was significantly attenuated by inhibiting this signal ((0.83±0.30)×10(4) μm(2) vs. (1.82±0.15)×10(4) μm(2,) P<0.05); positive autophagy makers LC3B and Beclin1 were detected in both agonist-CD137 group and anti-CD137 groups and the expression of LC3B and Beclin1 was substantially higher in anti-CD137 group. Western blot analysis indicated that the expression of LC3B and Beclin1 in agonist-CD137 group was significantly upregulated compared with the control group (0.17±0.01 vs. 0.03±0.08, P<0.05, and 0.12±0.02 vs. 0.06±0.02, P<0.05), which could be significantly downregulated in anti-CD137 group (0.28±0.09 vs. 0.17±0.01, P<0.05 and 0.17±0.02 vs. 0.12±0.02, P<0.05). TME showed that the number (QTY /HP) of autophagosome of agonist-CD137 group and anti-CD137 group in plaque were both increased (14.67±2.52 vs. 3.67±1.53, P<0.01, and 15.33±2.08 vs. 3.67±1.53, P<0.01), while in the agonist-CD137 group, the number of extracellular autophagosome within thoracic aortic atherosclerotic plaque of ApoE(-/-) mice increased more substantially (5.33±1.53 vs. 1.33±0.58, P<0.01). (2) In vitro study showed that activating CD137-CD137L signal could promote calcium deposition in extracellular matrix and the activity of osteogenesis phenotypic ALP((6.73±0.02) μmol/mg protein vs. (1.07±0.03) μmol/mg protein, P<0.05), and ((563.20±0.72) U/mg protein vs. (117.50±0.64) U/mg protein, P<0.05), while these effects were significantly blunted in anti-CD137 group ((1.94±0.05) μmol/mg protein vs. (6.73±0.02) μmol/mg protein, P<0.05, and (236.10±0.14) U/mg protein vs. (563.20±0.72) U/mg protein, P<0.05). TME showed that the number of intracellular autophagosome in agonist-CD137 group and anti-CD137 group was both significantly higher than in control group ((21.65±1.34) μg/ml vs. (8.32±1.58) μg/ml, P<0.01, and (15.42±1.65) μg/ml vs. (8.32±1.58) μg/ml, P<0.05). After the density gradient centrifugation, exocytotic autophagosome in the medium of agonist-CD137 group was markedly higher than in control group ((14.67±1.53) μg/ml vs. (2.33±1.15) μg/ml, P<0.01). (3) Compared with the control group, autophagosomes isolated from culture supernatant (final concentration: 15 μg/ml) could significantly stimulate calcium deposition((2.30±0.10) μmol/mg protein vs. (0.15±0.40) μmol/mg protein, P<0.05) and enhance the expression of bone morphogenetic protein 2 (2.10±0.04 vs. 0.30±0.01, P<0.05). Conclusion: CD137-CD137L signaling could mediate exocytosis of autophagosome within VSMCs, thus influence the formation of atherosclerotic calcification.
目的: 探讨CD137-CD137L信号通路是否通过调控自噬小体出胞影响动脉粥样硬化钙化形成。 方法: (1)在体实验:载脂蛋白E基因敲除(ApoE(-/-))小鼠15只,8周龄,雄性,采用随机数表法分为3组,即对照组、CD137激动组(腹腔注射激动型CD137抗体200 μg)、CD137抑制组(腹腔注射抑制型CD137抗体200 μg +激动型CD137抗体200 μg),每组5只,同时高脂喂养。采用Von Kossa染色法观察各组小鼠胸主动脉粥样硬化斑块钙化程度,免疫组织化学染色法观察斑块内自噬早中期标记物微管相关蛋白1轻链3B(LC3B)和酵母自噬基因Atg6的同源基因Beclin1的表达,Western blot法检测LC3B、Beclin1蛋白表达,透射电镜检测斑块中自噬小体形成。(2)细胞实验:采用组织块贴壁法培养C57BL/6J小鼠(基因背景与ApoE(-/-)小鼠一致)胸主动脉血管平滑肌细胞(VSMC),将细胞分为3组,即对照组、CD137激动组(激动型CD137抗体10 μg/ml加入培养基中)、CD137抑制组(抑制型CD137抗体10 μg/ml预处理细胞30 min后,加入激动型CD137抗体10 μg/ml于培养基),细胞外钙化分别采用Von Kossa染色和成骨表型碱性磷酸酶(ALP)活性检测。(3)出胞自噬小体的分离及分组干预:将细胞实验中CD137激动组细胞经相应处理获取自噬小体。取细胞实验中的小鼠VSMC予炎症因子白细胞介素-1β、干扰素-γ和肿瘤坏死因子-α各25 ng/ml刺激24 h后分为激动组(自噬小体终浓度为15 μg/ml)和对照组,检测两组钙盐沉积和成骨表型标志物骨形成蛋白2(BMP2)表达情况。 结果: (1)在体实验结果:CD137激动组小鼠胸主动脉粥样硬化斑块内钙化区域明显大于对照组(P<0.01),而CD137抑制组则小于CD137激动组(P<0.05)。CD137激动组和抑制组小鼠胸主动脉粥样硬化斑块内自噬标记物LC3B和Beclin1均为阳性表达,抑制组表达更为明显。Western blot结果显示CD137激动组LC3B表达水平高于对照组(P<0.05), CD137抑制组高于CD137激动组(P<0.05),CD137激动组Beclin1表达水平高于对照组(P<0.05), CD137抑制组高于CD137激动组(P<0.05)。透射电镜结果显示CD137激动组和抑制组小鼠胸主动脉粥样硬化斑块内自噬小体数量均多于对照组(P均<0.01)。(2)细胞实验结果:CD137激动组细胞外钙盐沉积量多于对照组(P<0.05),CD137抑制组则少于CD137激动组(P<0.05)。CD137激动组细胞成骨表型ALP活性高于对照组(P<0.05),CD137抑制组则低于CD137激动组(P<0.05)。透射电镜观察结果显示CD137激动组和抑制组细胞自噬小体含量均多于对照组(P<0.01或0.05),且密度梯度离心后显示CD137激动组培养液中出胞自噬小体含量明显多于对照组(P<0.01)。(3)出胞自噬小体分组干预结果:激动组VSMC细胞外钙盐沉积量明显多于对照组,胞浆中BMP2表达水平亦明显高于对照组(P均<0.05)。 结论: CD137-CD137L信号通路可通过介导自噬小体出胞调控动脉粥样硬化钙化形成。.
Keywords: Antigens, CD137; Atherosclerosis; Autophagy.