The role of adhesion molecules ICAM-1 and VCAM-1 in herpes simplex keratitis

Purpose:To elucidate the role of adhesion molecules in the pathogenesis of herpes simplex keratitis. Methods:Fifty female Balb/c mice (4-6 weeks old, 14-22 g weight) were divided into two groups randomly. Forty were infected by herpes simplex virus and the other 10 were used as normal controls.All mice were fed under the same conditions.Corneas of these mice were collected for immunohistochemical testing on day 14 and 21 after infection. Results:ICAM-1 was mainly expressed in the basal cells of the corneal epithelia and vascular endothelia of the infected mice. A substantial amount of VCAM-1 was also expressed in the corneal vascular endothelial cells of infected mice,and was also found in inflammatory cells in the epithelial and stromal layers of the corneas. Conclusion:Adhesion molecules ICAM-1 and VCAM-1 were involved in the progression of herpex simplex keratitis.They may accelerate the progress of inflammation by mediating the extravsation of inflammatory cells from vessels into the infected sites.

DNA vaccine expressing herpes simplex virus 1 glycoprotein C and D protects mice against herpes simplex keratitis

AIM： To investigate whether DNA vaccine encoding herpes simplex virus 1（HSV-1） glycoprotein C（g C） and glycoprotein D（g D） will achieve better protective effect against herpes simplex keratitis（HSK） than DNA vaccine encoding gD alone. METHODS： DNA vaccine expressing gD or gC combined g D（g D.g C） were constructed and carried by chitosan nanoparticle. The expression of fusion protein gD and gC were detected in DNA/nanoparticle transfected 293 T cells by Western-blot. For immunization, mice were inoculated with DNA/nanoparticle for 3 times with 2 wk interval, and two weeks after the final immunization, the specific immune responses and clinical degrees of primary HSK were evaluated. RESULTS： Fusion protein g D.g C could be expressed successfully in cultured 293 T cells. And, p RSC-g C.g DIL21 DNA/chitosan nanoparticle could effectively elicit strongest humoral and cellular immune response in primary HSK mice evidenced by higher levels of specific neutralizing antibody and s Ig A production, enhanced cytotoxicities of splenocytes and nature killer cells（NK）,when compared with those of gD alone or mocked vaccine immunized mice. As a result, gC-based vaccine immunized mice showed least HSK disease. CONCLUSION： gC-based DNA vaccine could effectively prevent the progress of primary HSK, suggesting that this DNA vaccine could be a promising vaccine for HSK treatment in the future.

Systemic IL-1β production as a consequence of corneal HSV-1 infection-contribution to the development of herpes simplex keratitis

This study sought to identify potential therapeutic targets in herpes simplex keratitis(HSK) patients with active and inactive infection by investigating peripheral cytokine production. Peripheral blood mononuclear cells(PBMCs) and serum were prepared from healthy controls and HSK patients during active infection or following treatment(inactive infection). Serum antibody titres were determined by ELISA. Protein expression levels were analysed by Western blot. Cytokine levels were determined by multiplex ELISA. Active corneal herpes simplex virus type 1(HSV-1) infection resulted in significantly elevated peripheral levels of IL-1β in HSK patients compared to healthy controls, and remained significantly increased following treatment. Elevated production of IL-1β in inactive patients was associated with significantly increased levels of IRF3 and STAT1, key proteins involved in promoting anti-viral immune responses. Our data suggest that inflammation persists beyond the period that it is clinically evident and that enhanced peripheral production of IL-1β may have implications for HSV-1 viral clearance in active and inactive HSK patients.

Herpes simplex virus-1 infection or Simian virus 40-mediated immortalization of corneal cells causes permanent translocation of NLRP3 to the nuclei

AIM: To investigate into the potential involvement of pyrin containing 3 gene(NLRP3), a member of the nucleotide-binding oligomerization domain-like receptors with cytosolic pattern recognition, in the host defense of corneas against viruses.METHODS: The herpes viral keratitis model was utilized in BALB/c mice with inoculation of herpes simplex virus-1(HSV-1). Corneal tissues removed during therapy of patients with viral keratitis as well as a Simian vacuolating virus 40(SV40)-immortalized human corneal epithelial cell line were also examined.Immunohistochemistry was used to detect NLRP3 in these subjects, focusing on their distribution in tissue or cells. Western blot was used to measure the level of NLRP3 and another two related molecules in NLPR3 inflammasome, namely caspase-1 and IL-1β.RESULTS: The NLRP3 activation induced by HSV-1infection in corneas was accompanied with redistribution of NLRP3 from the cytoplasm to the nucleus in both murine and human corneal epithelial cells. Furthermore,in the SV40-immortalized human corneal epithelial cells,NLRP3 was exclusively located in the nucleus, and treatment of the cells with high concentration of extracellular potassium(known as an inhibitor of NLRP3activation) effectively drove NLRP3 back to the cytoplasm as reflected by both immunohistochemistry and Western blot.· CONCLUSION: It is proposed that herpes virus infection activates and causes redistribution of NLRP3 to nuclei. Whether this NLRP3 translocation occurs with other viral infections and in other cell types merit further study.

Anti-viral activity of Staphylococcus aureus lysates against herpes simplex virus type-Ⅰinfection:an in vitro and in vivo study

AIM:To investigate the effect of Staphylococcus aureus(S.aures)lysates(SALs)on herpes simplex virus type-Ⅰ(HSV1)infection in human corneal epithelial(HCE)cells and in a mouse model of HSV1 keratitis.METHODS:HCE,Vero,HeLa,and BV2 cells were infected with HSV1[HSV1f strain,HSV1f;HSV-1-H129 with green fluorescent protein(GFP)knock-in,HSV1g].Pre-or post-infection,SAL at various concentrations was added to the culture medium for 24 h.GFP fluorescence in HSV1g or plaque formation by HSV1f were examined.The effects of heat-treated SAL,precooled acetone-precipitated SAL,and SAL subjected to ultrafiltration(100 kDa)were evaluated.The effects of other bacterial components and lysates on HSV1 infection were also tested,including lipoteichoic acid(LTA),peptidoglycan(PGN),staphylococcal protein A(SPA),andα-hemolysin from S.aureus(α-toxin)as well as lysates from a wild-type S.aureus strain,S.epidermidis,and Escherichia coli(W-SAL,SEL,and ECL,respectively).In addition,SAL eye drops were applied topically to BALB/c mice with HSV1 keratitis,followed by in vivo observations.RESULTS:The cytopathic effect,plaque formation(HSV1f),and GFP expression(HSV1g)in infected cells were inhibited by SAL in a dose-dependent manner.The active component of SAL(≥100 kDa)was heat-sensitive and retained activity after acetone precipitation.In HSV1ginfected cells,treatment with LTA-sa,α-toxin,PGN-sa,or SPA did not inhibit GFP expression.SAL,W-SAL,and SEL(but not ECL)decreased GFP expression.In mice with HSV1 keratitis,SAL reduced corneal lesions by 71%.CONCLUSION:The results of this study demonstrate that SAL can be used to inhibit HSV1 infection,particularly keratitis.Further studies are needed to determine the active components and mechanism underlying the effects of SAL.

Meta-Herpetic Keratitis and Therapeutic Approach: Case Report

The purpose of this study is to disclose the steps in the therapeutic approach for meta-herpetic corneal ulcer. Report of a case with anterior segment photography was used. The 6 months of follow-up results of the case were disclosed. The efficacy of the therapeutic approach for meta-herpetic corneal ulcer was discussed.

白介素2基因佐剂协同单纯疱疹病毒1型糖蛋白D核酸疫苗免疫诱导的特异性免疫应答

目的研究白介素2(IL-2)cDNA协同单纯疱疹病毒1型(HSV-1)gD核酸疫苗免疫对机体体液免疫和细胞免疫应答的影响,以及在HSV-1病毒角膜攻击时的保护效果。方法利用pcDNA3.1载体分别构建HSV-1糖蛋白D和IL-2的真核表达质粒pgD和pIL-2,体外鉴定其表达。动物实验分为pcDNA3.1空载体对照组、pgD单独免疫组和pgD+pIL-2联合免疫组3组,具体为通过肌肉免疫接种BALB/c小鼠3次,间隔2周,每次接种质粒100μg,第3次免疫后2周,用酶联免疫吸附试验(ELISA)检测抗体滴度并做亚型分析,利用3H-TdR掺入法进行Th细胞增殖实验,ELISA试剂盒检测Th细胞分泌的IL-2、IFN-γ和IL-10水平,耳廓肿胀实验检测迟发型超敏反应(DTH)反应;HSV-1病毒角膜攻击后,裂隙灯显微镜观察角膜上皮病变。结果与pgD单独免疫组相比,pIL-2的协同免疫可以显著提高IgG2a抗体滴度、Th细胞增殖反应和DTH反应,Th细胞分泌IL-2和IFN-γ水平也显著提高,IL-10水平明显下降。在动物保护实验中,pIL-2的协同免疫明显增强了pgD疫苗在病毒攻击时对角膜的保护效果。结论IL-2cDNA的协同免疫可以显著提高pgD核酸疫苗诱导的体液免疫和细胞免疫应答水平,增加核酸疫苗的免疫保护效果。

中西医结合治疗单纯疱疹病毒性角膜炎100例

目的:观察名老中医张望之先生经验方"清热退翳丸"联合1%阿昔洛韦滴眼液治疗单纯疱疹病毒性角膜炎的临床疗效。方法:将150例患者随机分为治疗组(100例)和对照组(50例),对照组予1%阿昔洛韦点眼,治疗组在对照组用药基础上予中药"清热退翳丸"内服。结果:治疗组治愈率和复发率分别为97%和7.14%,对照组的治愈率和复发率为92%和30.43%,两组相比治愈率无显著性差异(P>0.05),复发率有显著性差异(P<0.05);疗程时间两组相比有显著性差异(P<0.05)。结论:对单纯疱疹病毒性角膜炎,采用中药清热退翳丸联合西药1%阿昔洛韦滴眼液治疗见效快,复发率低。

DNA疫苗pRSC-gD.gC-IL-21的构建及其预防HSK的动物实验初步研究

目的:构建DNA疫苗pRSC-gD.gC-IL-21,探讨其是否能诱导动物免疫应答及抵抗眼角膜单纯疱疹病毒Ⅰ型(HSV-1)的感染。方法:提取HSV-1基因组DNA,PCR扩增获得gC基因。以pRSC-gD-IL-21质粒为模板(本实验室2011年构建),构建重组质粒pRSC-gD.gC-IL-21,用纳米材料壳聚糖(chitosan)包裹,采用黏膜接种的方式分别以pRSC-gD.gC-IL-21+chitosan、pRSC-gD-IL-21+chitosan、pRSC+chitosan及chitosan免疫小鼠3次,间隔2周,末次免疫2周后检测各项免疫学指标,同时评价小鼠对病毒攻击角膜的免疫保护作用。结果:经测序、酶切及Westernblot鉴定,重组质粒pRSC-gD.gC-IL-21构建成功,chitosan包裹率高。与对照鼠相比,该疫苗在鼠体内产生了更强的特异性中和抗体、细胞毒性T淋巴细胞(CTL)及自然杀伤细胞(NK)杀伤活性增强、泪液中特异性sIgA水平增高,同时使小鼠产生了较强的针对眼角膜HSV-1感染的免疫保护作用。结论:DNA疫苗pRSC-gD.gC-IL-21构建成功,能诱导小鼠产生较强的免疫应答及针对HSV-1眼部感染的免疫保护作用,能够预防单纯疱疹病毒性角膜炎(HSK)的发生、发展。

Irf3基因缺失导致角膜组织对HSV-1病毒易感性增强

目的研究IRF3缺失对单纯疱疹性角膜炎的发病进程影响以及病理学依据。方法用HSV-l感染对照组和实验组小鼠角膜,同时用培养基(不含病毒)处理Irf3^(-/-)小鼠角膜作为溶剂对照组。分别用裂隙灯显微镜、HD-OCT、角膜共聚焦技术观察各组角膜的临床变化;采用组织学技术检查角膜病理学改变;用QRT-PCR检测角膜中HSV-1的表达水平;用蛋白免疫印迹法检测炎性指标在各组角膜组织中的表达水平。用流式细胞术、全身症状记录观察小鼠全身感染情况。结果实验组角膜接种HSV-1后第7天开始出现角膜上皮缺损等角膜基质炎早期症状,并且逐渐加重,发病率持续增高。对照组发病率显著较低,且症状比实验组明显减轻。Irf3^(-/-)溶剂对照组无明显角膜感染变化。QRT-PCR和蛋白免疫印迹法结果显示,实验组HSV-1、IL-9、IL-10、IL-18、TNF-α表达水平均比对照组、Irf3^(-/-)溶剂对照组显著较高。脾脏流式细胞术、全身症状记录结果显示实验组比对照组、Irf3^(-/-)溶剂对照组全身炎性反应明显较重,提示有全身感染。结论 IRF3是角膜HSV-1感染的重要感受信号分子,它的缺失使小鼠发生单纯疱疹病毒性角膜炎的易感性明显增高。

羊膜移植对实验性HSK中基质金属蛋白酶表达的影响

目的研究羊膜移植(AMT)对单纯疱疹性角膜炎(HSK)中基质金属蛋白酶(MMP-2,-9)表达的影响。方法40只BALB/c小鼠角膜感染Ⅰ型单纯疱疹病毒(HSV-1),实验组角膜行AMT。术后第0、2、7、14 d取出角膜。常规病理切片、免疫组化染色和计算机图像分析检测角膜中MMP-2及-9的表达及平均光度值的变化。结果对照组20只鼠眼中17只发生HSK;AMT组仅有9只眼发生,差异有显著统计学意义(P<0.01)。AMT组角膜上皮、基质病变程度及新生血管发生率明显低于对照组(P<0.05)。免疫组化及图像分析显示对照组角膜细胞和浸润炎性细胞中表达的MMP-2及-9在第2 d增加,14 d时达高峰。AMT组各时间点MMP-2及-9表达低于对照组,差异有显著统计学意义(P<0.05)。结论羊膜移植可能通过抑制角膜细胞及浸润的炎症细胞产生MMPs,从而抑制HSK的发生和发展。

无环鸟苷抑制小鼠单纯疱疹性角膜炎潜伏病毒激活作用的研究

目的 证实无环鸟苷能够作用于潜伏单疱病毒的激活阶段 ,抑制病毒活化。方法 以Balb/c小鼠作为潜伏感染模型 ,以紫外线B照射为激活条件 ,治疗组给予无环鸟苷口服 ,停药后 1天处死动物检测活化病毒。结果 治疗组3 0例中无 1例 ,而对照组 3 0例中有 12例检测出活化病毒 (P <0 0 1) ;治疗至照射后 2天的 10只鼠无 1例 ,而相应对照组 10只中 6例检出活化病毒 (P <0 0 1)。结论 预防性应用ACV特异作用于病毒激活期 ,有效的抑制病毒活化。

白细胞介素-9在单纯疱疹病毒性角膜基质炎小鼠角膜组织中的表达

背景单纯疱疹病毒性角膜基质炎（HSK）是一种由CD4＋T淋巴细胞介导的免疫病理性疾病。国外研究发现，白细胞介素一9（IL一9）在多种免疫性疾病的发病过程中发挥重要作用，但在HSK中是否起作用目前少有报道。目的研究小鼠HSK发生和发展过程中IL一9在角膜组织中的表达，探讨IL一9的表达与HSK进展程度之间的关系。方法4～6周龄清洁级健康BALB／c小鼠180只分为对照组20只和实验组160只。对照组仅进行“#”字形划痕，不接种病毒；实验组小鼠角膜用注射针划痕后接种5μl含有1×10^6空斑单位（PFU）／ml的I型单纯疱疹病毒（HSV-1）KOS毒株建立HSK小鼠模型。分别于病毒接种前（0d），接种后1、3、5、7、8、10、14、21d在裂隙灯显微镜下观察小鼠角膜的变化；于接种后14d制备角膜组织切片，苏木精一伊红染色观察角膜的组织病理学改变；采用荧光实时定量PCR（real-timePCR）法检测IL-9mRNA在小鼠角膜组织中的表达；采用免疫荧光组织化学方法检测IL-9蛋白在小鼠角膜组织中的表达。结果裂隙灯显微镜下观察结果显示，小鼠角膜接种HSV-1后第3天，实验组小鼠出现点状、树枝状、地图状角膜上皮缺损，接种后6d内上皮缺损痊愈，但于接种后第7天起出现角膜基质灰白色混浊，14d基质混浊加重并达高峰，之后逐渐减轻。Real—timePCR结果显示，未接种病毒（0d）的正常小鼠角膜组织中仅有极微量的IL-9mRNA表达，实验组小鼠接种病毒后1、3、5、7、8、10、14dIL-9mRNA在角膜组织中的相对表达量分别为6．37±0．45、5．66±0．53、3．93±0．35、5．62±0．34、3．23±0．18、2．57±0．14、2．19±0．20，总体表达差异有统计学意义（F=92．764，P=0．000），其中接种后各时间点IL-9mRNA相对表达量与0d比较明显增高，差异均有统计学意义（P〈0．05），接种病毒后21d，IL-9mRNA相对表达量与0d比较差异无统计学意义（P=0．340）。免疫荧光组织化学法检测显示，IL-9蛋白在实验组小鼠角膜的上皮层、基质层及内皮细胞层呈强阳性表达，而对照组小鼠角膜组织中未见IL-9蛋白的表达。结论采用角膜划痕和HSV-1KOS毒株接种法可成功建立BALB／c小鼠HSK模型，IL-9参与了HSK的免疫炎症反应。

实验性单纯疱疹性角膜炎的免疫组织化学研究

目的 研究单纯疱疹Ⅰ型病毒 (HSV 1)感染后疾病的严重性与宿主遗传因素的关系 ;分析HSV 1感染后小鼠角膜中炎症细胞的亚群分布 ;检测角膜三层细胞中病毒抗原的表达及其临床意义。方法 以单克隆抗体和常规组织学技术作免疫组织化学研究。结果 HSV 1感染后疾病取决于宿主的遗传因素 ,在角膜基质炎中 ,T细胞对引发疾病起主导作用 ,炎症细胞的数量与抗原量相关 ,病毒抗原沉积于角膜三层细胞 ,而BLAB/c中的频率 ( 71%～ 10 0 % )高于C5 7BL/ 6( 11%～ 5 6% )。结论 实验性单纯疱疹性角膜基质炎的严重性取决于宿主的遗传因素 :在引发角膜基质炎过程中 ,T细胞起主导作用 ;基质层为HSV 1最主要沉积场所 。

用“红细胞免疫检测法”研究单疱病毒性角膜炎病人细胞免疫功能的变化

用先进的“红细胞免疫检测法”测定正常人及单疱病毒性角膜炎患者应用单疤病毒特异性转移因子（ＨＳＶ─ＩＴＦ）治疗前后红细胞免疫功能，其结果：１０例正常人与５０例治疗前病人比较（Ｐ＜０．０１），两组有显著性差异。５０例治疗前与２０例治疗后病人比较（Ｐ＜０．０１），两组有显著性差异。表明ＨＳＫ病人治疗前免疫功能明显低下，用ＨＳＶ─ＩＴＦ治疗后，红细胞免疫功能显著提高。

单纯疱疹病毒性角膜基质炎的鼠模型建立

目的 建立单纯疱疹病毒性角膜基质炎 (HSK)的鼠模型 ,为研究HSK的发病机制及临床治疗奠定基础。方法 用HSV 1RE株感染Balb c鼠角膜 ,建立HSK的鼠模型 ,并在感染后 1天、3天、7天观察病变。结果 实验组鼠角膜有HSK病变发生 ,而空白对照组鼠角膜上皮愈合、完整光滑。结论 HSV 1RE株感染Balb c鼠有效 ,可致HSK发生。

基于热、药分离方式的明目解毒方熏蒸对兔单纯疱疹病毒性角膜炎影响的实验研究

目的采用热、药分离的方式探讨明目解毒方熏蒸对于单纯疱疹病毒性角膜炎(HSK)的作用途径。方法90只健康新西兰大白兔采用随机数字表法分为正常对照组、模型组、中药熏蒸组、热熏蒸组和熏蒸液组5组,每组18只。除正常对照组外,其余各组均采用眼表划痕法给予单纯疱疹病毒I型(HSV-1)接种建立HSK模型。造模后模型组和正常对照组不予药物处理,中药熏蒸组采用明目解毒方每日熏蒸干预,热熏蒸组采用蒸馏水熏蒸,熏蒸液组采用明目解毒方熏蒸液滴眼。分别于造模前1 d和造模1 d、3 d、7 d,对各组实验兔的角膜病变程度进行评分。并在治疗1 d、3 d、7 d随机抽取每组6只眼,采用PCR法检测角膜组织中HSV-1的表达,ELISA法检测房水中IL-2和IFN-γ的含量;采用Western blot方法检测外周血中CD4、CD8的蛋白表达情况。结果治疗3 d、7 d,中药熏蒸组、熏蒸液组和热熏蒸组的兔角膜HSV-1含量低于模型组(P<0.05);各组间房水中IFN-γ的含量差异无统计学意义(P>0.05),治疗7 d,中药熏蒸组和热熏蒸组存在交互作用。治疗1 d、3 d、7 d,中药熏蒸组房水中IL-2含量与模型组差异有统计学意义(P<0.05);治疗1 d、7 d熏蒸液组与模型组房水中IL-2含量差异有统计学意义(P<0.05)。治疗3 d、7 d中药熏蒸组较模型组外周血CD4蛋白表达明显增强(P<0.05)。结论明目解毒方熏蒸可通过热、药效应清除HSK角膜组织中的HSV-1病毒,并且影响局部免疫因子IL-2水平,上调外周血CD4的表达。

单纯疱疹病毒性角膜炎治疗方法研究进展

单纯疱疹病毒1型(herpes simplex virus 1, HSV-1)是一种普遍存在的病原体,感染角膜可引起单纯疱疹病毒性角膜炎(herpes simplex keratitis, HSK)。HSV-1可潜伏于三叉神经胞体,易形成复发感染。多次反复恶化可造成角膜免疫-炎症反应损伤,促进新生血管形成,进一步导致角膜浑浊、视力障碍甚至失明,是导致角膜盲的首要病因之一。目前,临床使用的抗病毒药物不能根除HSV-1,本文将汇总有关HSK的最新治疗进展,主要从抑制HSV-1入侵、增殖以及减少新血管生成两方面进行综述,以期为临床研究提供理论依据。

HSV-gD-IL-21 DNA疫苗免疫效应及抗鼠眼角膜HSV-1感染的初步研究

构建共表达HSV-1型gD和鼠源性IL-21DNA疫苗,探讨其是否能诱导动物免疫应答以及抵抗眼角膜HSV-1的感染。PCR扩增HSV-1gD和IL-21基因,分别定向插入载体pRSC中,构建DNA疫苗pRSC-gD-IL-21,对其进行鉴定后再分别以pRSC-gD-IL-21、pRSC-gD、pRSC免疫小鼠3次,间隔2周,末次免疫2周后检测血清抗体、IL-4及IFN-γ水平,特异性脾细胞增殖反应以及CTL、NK细胞杀伤活性。同时评价小鼠对病毒攻击角膜的免疫保护作用。经测序、酶切和RT-PCR鉴定后表明,pRSC-gD-IL-21中目的基因在细胞内成功转录表达。与对照鼠相比,该疫苗在鼠体内产生了较强的特异性抗体、IL-4及IFN-γ、特异性脾细胞增殖反应、CTL及NK细胞杀伤活性均增强,同时疫苗使小鼠产生了较强的针对眼角膜HSV-1感染免疫保护作用。结果显示,pRSC-gD-IL-21疫苗能诱导小鼠产生较强的免疫应答及针对HSV-1眼部感染的免疫保护作用。

单纯疱疹病毒1型(HSV-1)糖蛋白B基因疫苗对HSV-1原发及潜伏感染的抑制作用

目的观察单纯疱疹病毒1型（herpes simplex virus-1,HSV-1）糖蛋白B基因疫苗（pg B）在防治HSV-1原发及潜伏感染的作用。方法将BALB/c小鼠随机分为4组：A组（实验组,注射含质粒pg B的PBS）、B组（阳性对照组,注射灭活的HSV-1病毒液）、C组（载体对照组,注射含质粒pc DNA3的PBS）和D组（空白对照组,注射PBS）。各组小鼠均于双侧股四头肌多点注射,共免疫3次,间隔3周。于末次免疫3周后行角膜划痕接种HSV-1。术后1～14、21和28 d行角膜荧光素染色,在裂隙灯显微镜下观察角膜炎病变形成情况。角膜接种病毒第30天,处死全部小鼠,取三叉神经节,接种Vero细胞,观察病毒潜伏感染形成情况。结果 A组和B组小鼠接种HSV-1后仅有轻度角膜上皮炎发生,且6 d内全部愈合,组间比较差异无统计学意义（P〉0.05）;C组和D组小鼠接种后第2天角膜上皮炎达到高峰,7 d后炎症慢慢消失,与A组比较,差异有统计学意义（P〈0.05）。A组和B组小鼠接种后未发生角膜基质炎,且无1例死亡;C组和D组小鼠在接种后第5天出现炎症反应,并逐渐加重,接种后11～14 d角膜基质炎达到高峰,在接种后第30天有30%小鼠死亡。Vero细胞检测病毒潜伏感染,A组和B组未发生细胞病变,而C组和D组第5天发生细胞病变。结论 pg B能有效预防实验小鼠HSV-1原发感染,并抑制潜伏感染的形成。