抗CD40L抗体免疫调节对小鼠眼前节腺病毒介导的转基因表达的影响。
Effect of immunomodulation with anti-CD40L antibody on adenoviral-mediated transgene expression in mouse anterior segment.
作者信息
Millar J Cameron, Pang Iok-Hou, Wang Wan-Heng, Wang Yu, Clark Abbot F
机构信息
Alcon Research, Ltd., Fort Worth, TX 76134, USA.
出版信息
Mol Vis. 2008 Jan 9;14:10-9.
PURPOSE
Gene transduction using adenoviral vectors is an important research tool. To assess and optimize this technique for glaucoma research, we characterized green fluorescent protein (GFP) expression in the mouse eye after intraocular injection of adenoviral vector encoding GFP (Ad5.CMV-GFP) and evaluated the effect of anti-CD40L antibody administration on GFP expression.
METHODS
Mice were injected with Ad5.CMV-GFP intracamerally (IC) or intravitreally (IVT) with or without anti-CD40L antibody treatment. GFP expression was assessed by in vivo fluorescence intensity with a standardized grading scale. Location of expression was analyzed histologically by fluorescence microscopy.
RESULTS
Intraocular injection of Ad5.CMV-GFP induced titer-dependent expression of GFP in the anterior segment. In vivo fluorescence was detectable but low after IC injection. After IVT injection, fluorescence in the eye peaked at days 4-7 with a fluorescence grade of 3.0 +/-0.0 (mean +/-SEM, n=6; injection with 1x10(8) pfu vector). After day 7, GFP expression declined significantly. Treatment with anti-CD40L antibody increased fluorescence intensity after IC injection, and prolonged GFP expression in the IVT group. At day 43, fluorescence grades of the IVT group were 2.8 +/-0.7 (with anti-CD40L) and 1.2 +/-0.6 (without antibody). Three-Way ANOVA confirmed that GFP expression was significantly higher in the anti-CD40L than the no antibody group (p=0.013), significantly higher in the IVT than the IC group (p=0.003), and significantly higher in the high viral titer (1x10(8) pfu) than the low titer (1x10(7) pfu) group (p=0.010). Fluorescence microscopic examination of cross-sections of eyes indicated GFP expression in the trabecular meshwork (TM), corneal endothelium, and sporadically iris, ciliary body and lens epithelium.
CONCLUSIONS
Intraocular injection of Ad5.CMV-GFP induced GFP expression in the mouse anterior segment, including the TM. Expression was more prominent after IVT injection than IC injection. Anti-CD40L antibody treatment increased both intensity and duration of GFP expression. These findings provide important and practical means to improve duration and efficiency of adenovirus-mediated transgene expression in the eye.
目的
使用腺病毒载体进行基因转导是一种重要的研究工具。为了评估和优化该技术用于青光眼研究,我们对编码绿色荧光蛋白(GFP)的腺病毒载体(Ad5.CMV-GFP)眼内注射后小鼠眼中GFP的表达进行了特征分析,并评估了给予抗CD40L抗体对GFP表达的影响。
方法
对小鼠进行前房内(IC)或玻璃体内(IVT)注射Ad5.CMV-GFP,同时给予或不给予抗CD40L抗体治疗。通过标准化分级量表的体内荧光强度评估GFP表达。通过荧光显微镜进行组织学分析以确定表达位置。
结果
眼内注射Ad5.CMV-GFP在前房诱导了GFP的滴度依赖性表达。IC注射后可检测到体内荧光,但强度较低。IVT注射后,眼部荧光在第4至7天达到峰值,荧光等级为3.0±0.0(平均值±标准误,n = 6;注射1×10⁸ pfu载体)。第7天后,GFP表达显著下降。抗CD40L抗体治疗增加了IC注射后的荧光强度,并延长了IVT组中GFP的表达。在第43天,IVT组的荧光等级为2.8±0.7(使用抗CD40L)和1.2±0.6(不使用抗体)。三因素方差分析证实,抗CD40L组的GFP表达显著高于无抗体组(p = 0.013),IVT组显著高于IC组(p = 0.003),高病毒滴度(1×10⁸ pfu)组显著高于低滴度(1×10⁷ pfu)组(p = 0.010)。眼部横断面的荧光显微镜检查表明,小梁网(TM)、角膜内皮以及偶尔在虹膜、睫状体和晶状体上皮中有GFP表达。
结论
眼内注射Ad5.CMV-GFP可在小鼠前房包括TM诱导GFP表达。IVT注射后的表达比IC注射更明显。抗CD40L抗体治疗增加了GFP表达的强度和持续时间。这些发现为提高腺病毒介导的转基因在眼内表达的持续时间和效率提供了重要且实用的方法。
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