Kim Jong-Mook, Lim Byung-Kwan, Ho Seong-Hyun, Yun Soo-Hyeon, Shin Jae-Ok, Park Eun-Min, Kim Duk-Kyung, Kim Sunyoung, Jeon Eun-Seok
ViroMed Co. Ltd, Seoul, Republic of Korea.
Biochem Biophys Res Commun. 2006 Jun 9;344(3):765-71. doi: 10.1016/j.bbrc.2006.03.170. Epub 2006 Apr 5.
Tumor necrosis factor-alpha (TNF-alpha) is one of the major cytokines that modulate the immune response in viral myocarditis, but its role has not yet been thoroughly evaluated. We antagonized TNF-alpha using the expressed soluble p75 TNF receptor linked to the Fc portion of the human IgG1 gene (sTNFR:Fc) by in vivo electroporation, and evaluated its effects on experimental coxsackieviral B3 (CVB3) myocarditis. A plasmid DNA encoding sTNFR:Fc (15microg/mouse) was injected into the gastrocnemius muscles of Balb/C male mice followed by electroporation (day -1). Control mice were injected with an empty vector. One day after electroporation, mice were infected with CVB3 (day 0). Serum levels of sTNFR:Fc increased from day 2 and peaked at day 5 following electroporation. The heart virus titers of sTNFR:Fc mice were higher than those of controls at day 3. However, subsequent to day 12, the survival rates of the sTNFR:Fc mice were significantly higher than those of the controls (36% versus 0% at day 27, P<0.01). Histopathological examination indicated that inflammation and myocardial fibrosis were significantly decreased in sTNFR:Fc mice at day 12. The expressed sTNFR:Fc could modulate the inflammatory process during the post-viremic phase of viral myocarditis.
肿瘤坏死因子-α(TNF-α)是调节病毒性心肌炎免疫反应的主要细胞因子之一,但其作用尚未得到充分评估。我们通过体内电穿孔法,使用与人类IgG1基因Fc部分相连的表达可溶性p75 TNF受体(sTNFR:Fc)来拮抗TNF-α,并评估其对实验性柯萨奇病毒B3(CVB3)心肌炎的影响。将编码sTNFR:Fc(15μg/小鼠)的质粒DNA注射到Balb/C雄性小鼠的腓肠肌中,随后进行电穿孔(第-1天)。对照小鼠注射空载体。电穿孔后一天,小鼠感染CVB3(第0天)。电穿孔后第2天血清sTNFR:Fc水平开始升高,并在第5天达到峰值。在第3天,sTNFR:Fc小鼠的心脏病毒滴度高于对照组。然而,在第12天之后,sTNFR:Fc小鼠的存活率显著高于对照组(第27天为36%对0%,P<0.01)。组织病理学检查表明,在第12天,sTNFR:Fc小鼠的炎症和心肌纤维化明显减轻。表达的sTNFR:Fc可调节病毒性心肌炎病毒血症后阶段的炎症过程。
