Black Garlic as an Antiviral for Herpes Simplex Virus-2 in Lung Cells

Allicin, an antioxidant, is known for providing garlic with its unique fragrance and taste, as well as for its antimicrobial properties. Black garlic, a fermented form of garlic, contains higher levels of antioxidants than fresh garlic. Antioxidants play a vital role in alleviating cellular stress during viral infections. Viral infections result in oxidative stress through the production of reactive oxidative species (ROS). A prolonged state of oxidative stress can result in cell death, DNA damage, and disease progression. In this study, black garlic extract (BGE) is evaluated for its ability to mitigate cytopathic effects and oxidative stress caused by herpes simplex virus-2 (HSV-2) infections in vitro. Antiviral assays were performed to determine the percent of viral inhibition resulting from treatment with the BGE. ROS-GloTM H2O2 assays were then completed to measure the post-infection ROS levels of BGE-treated virus and cells. The results thus far suggest that BGE may inhibit viral infection and decrease levels of oxidative stress.

Antiviral activity of Basidiomycete mycelia against influenza type A(serotype H1N1) and herpes simplex virus type 2 in cell culture

In this study, we investigated the in vitro antiviral activity of the mycelia of higher mushrooms against influenza virus type A(serotype H1N1) and herpes simplex virus type 2(HSV-2), strain BH. All 10 investigated mushroom species inhibited the reproduction of influenza virus strain A/FM/1/47(H1N1) in MDCK cells reducing the infectious titer by 2.0–6.0 lg ID50. Four species, Pleurotus ostreatus, Fomes fomentarius, Auriporia aurea, and Trametes versicolor, were also determined to be effective against HSV-2 strain BH in RK-13 cells, with similar levels of inhibition as for influenza. For some of the investigated mushroom species—Pleurotus eryngii, Lyophyllum shimeji, and Flammulina velutipes—this is the first report of an anti-influenza effect. This study also reports the first data on the medicinal properties of A. aurea, including anti-influenza and antiherpetic activities. T. versicolor 353 mycelium was found to have a high therapeutic index(324.67), and may be a promising material for the pharmaceutical industry as an anti-influenza and antiherpetic agent with low toxicity. Mycelia with antiviral activity were obtained in our investigation by bioconversion of agricultural wastes(amaranth flour after CO2 extraction), which would reduce the cost of the final product and solve some ecological problems.

SEARCH FOR HERPES SIMPLEX VIRUS TYPE2（HSV－2）AND HUMAN PAPILLOMAVIRUS（HPV）IN THE NORMAL AND ABNORMAL CERVICAL SAMPLES

The specimens of 111 cervical carcinomas. 68 chronic cervicitis and 43 normal cervical exfoliated epithelial cells were examined for the presence of HSV2 DNA sequences with DNA hybridization using HSV2 BgL Ⅱ N fragment probe labelled by 32PdCTP. The result showed that the infection rates of HSV2 in the samples of cervical cancer.chronic cervicitis and normal epithelial cells were 1 4. 41 %(16/111). 27.94%( 19/68) and 25.58% ( 11/43),respectively. It was implied that early stages carcinogenesis of cervical epithelial cells might be correlated with the HSV2 infection.Sixteen HSV 2 positive samples of cervical carcinomas were also examined for the presence of the sequences homologous to human papillomavirus (HPV) type 6B/11. 16 and 18 DNA using dot blot hybridization (Tm17℃). The result indicated that 13 out of 16 were HPV 16 DNA hybridization positive accounting for 81. 2% of all HSV-2 positive samples and none of them were positive for HPV type 6B/11 and 18. The result indicated that double infection of HSV 2 and HPV16 in the same cervical carcinoma tissues may provide a strong evidence of the viral synergistic interaction in the induction of female cervical

FAILURE OF HERPES SIMPLEX VIRUS TYPE 2 TO SUBSTITUTE FOR DIMETHYL-BENZANTHRACENE IN TWO-STAGE SKIN CARCINOGENESIS

There are some Indications thtt herpes aimplex virus (HSV) may be mutagenic. Specific chromosomal changes have also been demonstrated In cultured cells infected with HSV. To further Investigate the mutagenic activity of HSV type 2 (HSV-2) we used mouse skin as a model system for cardnogenetls. Inoculation of the back skin of 4-week-old Sencar mke with live virus twice per week for one week or with Inactivated virus twice per week for two weeks was used to Initiate the mouse akin. After Initiation with HSV-2, 12-O-tetradecanoylphorbol-13-acetale(TPA) was applied twice weekly for 50 weeks as a promoter. During a period of 52 weeks, no skin carcinoma was found In the experimental groups, whereas 55% of control mice treated with 9, 10-dlmethy1-1, 2- benzanthracene (DMBA ) and then with TPA-developed skin carcinoma. The results demonstrate that HSV-2 could not substitute for DMBA in this animal model of two-stage skin carcinogenesis.

Human Herpes Virus Type 2 ( HSV2 ), Human Cytomegalovirus (HCMV) in the Male Genital Tract and Fertilization

The possibility of infection of the human male genital tract by human herpes virus type 2 (HSV2) or human cytomegalovirus (HCMV) is well established and their sexual transmission has been the object of many studies. Moreover, medically assisted procreation, which helps in numerous fertility problems, raises the question of new viral risks linked to the application of these new technologies. In this review, we shall consider current knowledge in terms of the presence of HSV 2 and HCMV in the different parts of the genital tract of immunocompetent or immunodepressed men. We shall also consider the possibility of viral transmission by the sexual act or by the various techniques used in medically assisted procreation. We shall describe studies in human beings and in animals.

Anti-herpes simplex virus activities of monogalactosyl diglyceride and digalactosyl diglyceride from Clinacanthus nutans, a traditional Thai herbal medicine

Objective: To evaluate the monogalactosyl diglyceride(MGDG) and digalactosyl diglyceride(DGDG) from Clinacanthus nutans(C. nutans) for their in vitro antiviral activities against herpes simplex virus type 1(HSV-1) and type 2(HSV-2) by plaque reduction assay.Methods: MGDG and DGDG were extracted with chloroform from C. nutans leaves.MGDG and DGDG were separated from chloroform crude extract using column chromatography, characterized by thin layer chromatography and quantified by high performance liquid chromatography. The anti HSV-1 and 2 activity against pre-treatment and posttreatment of the compounds was evaluated using plaque reduction assay. The cytotoxicity of the extract and the compounds on Vero cells were performed by MTT assay.Results: MGDG and DGDG obtained by column chromatography showed identical profiles as standard MGDG and standard DGDG using thin layer chromatography and high performance liquid chromatography. MGDG and DGDG from C. nutans showed 100%inhibition of HSV-1 replication at the post step of infection at noncytotoxic concentration with IC50 values of 36.00 and 40.00 mg/m L, and HSV-2 at 41.00 and 43.20 mg/mL,respectively. Moreover, MGDG and DGDG from C. nutans were demonstrated to have antiherpes simplex activity at the same level as standard synthetic compounds. In contrast, pretreatment of Vero cells with MGDG and DGDG before HSV-1 and HSV-2 infection did not show inhibitory effect against these viruses. MGDG and DGDG exhibited antiviral activity against HSV-1 with selectivity index of 26.00 and 23.00 and HSV-2 of 23.30 and 21.30.Conclusions: MGDG and DGDG from C. nutans, a traditional Thai herbal medicine illustrated inhibitory activity against HSV-1 and HSV-2, probably by inhibiting the late stage of multiplication, suggesting their promising use as anti-HSV agents.

Construction of the recombinant vector carrying herpes simplex virus thymidine kinase and cytokine genes expressed in cell line Tca8113

Objective: To construct expression vector containing fusion genes of herpes simplex virus thymidine kinase(Hsv-tk), Interleukin-2(IL-2) with internal ribosome entry sites(IRES), and to assess their expression in cell line Tca8113. Methods: IL-2 cDNA was obtained by reverse transcription. Hsv-tk, IL-2 and IRES genes were amplified by PCR. The purified amplification products were inserted into pGEM-T-Easy, and transformed into E.coli JM109. The purified recombinant plasmids were identified by restriction endonucleases. The recombinant plasmids were digested and pEGFP-N 3 were linearized, DNA fragments of Hsv-tk, IRES and IL-2 were ligated into linearized pEGFP-N 3, and then transferred into E.coli JM109. The recombinant tk-IL-2 genes were cloned separately and introduced into the expression vector pEGFP-N 3 containing GFP. The recombinant vectors were identified by their restriction sites through PCR. The plasmids pEGFP-TI was also transfected into Tca8113 cells by calcium phosphate method for the expression of fusion proteins. Fusion genes expressing vector PL(TI)SN was generated by the fusion of HSV-tk, IRES and IL-2 with the use of DNA recombination technology. The recombinant retroviruses were transferred into Tca8113 cells by lipofectamine. The positive clones were obtained after G418 selection and named Tca/TI respectively. Results: The pEGFP-TI pasmid was identified respectively by restriction endonucleases, and their fragment sizes were 1 120 bp and 450 bp. The pEGFP-TI pasmid as templates were amplified respectively by PCR, and their PCR products were 1 120 bp and 450 bp. The pEGFP-TI vectors were used to transfect Tca8113 cell, and the cells with fluorescence accounted for 60% of the total amount. Conclusion: pFGFP-tk-IRES-IL-2 expressing vector is easy to assess the expression of tk-IRES-IL-2-GFP fusion protein localization in transfected cells. The successful construction of expressing vector containing fusion genes of Hsv-tk, IRES and IL-2 may be beneficial for gene therapy in cell line Tca8113.

Construction and characterization of a synthesized herpes simplex virus H129-Syn-G2

Herpes simplex virus type 1(HSV-1)causes lifelong infections worldwide,and currently there is no efficient cure or vaccine.HSV-1-derived tools,such as neuronal circuit tracers and oncolytic viruses,have been used exten-sively;however,further genetic engineering of HSV-1 is hindered by its complex genome structure.In the present study,we designed and constructed a synthetic platform for HSV-1 based on H129-G4.The complete genome was constructed from 10 fragments through 3 rounds of synthesis using transformation-associated recombination(TAR)in yeast,and was named H129-Syn-G2.The H129-Syn-G2 genome contained two copies of the gfp gene and was transfected into cells to rescue the virus.According to growth curve assay and electron microscopy results,the synthetic viruses exhibited more optimized growth properties and similar morphogenesis compared to the parental virus.This synthetic platform will facilitate further manipulation of the HSV-1 genome for the devel-opment of neuronal circuit tracers,oncolytic viruses,and vaccines.

The Chinese herbal prescription JieZe-1 inhibits caspase-1-dependent pyroptosis induced by herpes simplex virus-2 infection in vitro

Objective:JieZe-1(JZ-1),a Chinese herbal prescription,has an obvious effect on genital herpes,which is mainly caused by herpes simplex virus type 2(HSV-2).Our study aimed to address whether HSV-2 induces pyroptosis of VK2/E6E7 cells and to investigate the anti-HSV-2 activity of JZ-1 and the effect of JZ-1 on caspase-1-dependent pyroptosis.Methods:HSV-2-infected VK2/E6E7 cells and culture supernate were harvested at different time points after the infection.Cells were co-treated with HSV-2 and penciclovir(0.078125 mg/mL)or caspase-1 inhibitor VX-765(24 h pretreatment with 100μmol/L)or JZ-1(0.078125-50 mg/mL).Cell counting kit-8 assay and viral load analysis were used to evaluate the antiviral activity of JZ-1.Inflammasome activation and pyroptosis of VK2/E6E7 cells were analyzed using microscopy,Hoechst 33342/propidium iodide staining,lactate dehydrogenase release assay,gene and protein expression,coimmunoprecipitation,immunofluorescence,and enzyme-linked immunosorbent assay.Results:HSV-2 induced pyroptosis of VK2/E6E7 cells,with the most significant increase observed 24 h after the infection.JZ-1 effectively inhibited HSV-2(the 50%inhibitory concentration=1.709 mg/mL),with the 6.25 mg/mL dose showing the highest efficacy(95.76%).JZ-1(6.25 mg/mL)suppressed pyroptosis of VK2/E6E7 cells.It downregulated the inflammasome activation and pyroptosis via inhibiting the expression of nucleotide-binding oligomerization domain-like receptor family pyrin domaincontaining protein 3(P<0.001)and interferon-γ-inducible protein 16(P<0.001),and their interactions with apoptosis-associated speck-like protein containing a caspase recruitment domain,and reducing cleaved caspase-1 p20(P<0.01),gasdermin D-N(P<0.01),interleukin(IL)-1β(P<0.001),and IL-18 levels(P<0.001).Conclusion:JZ-1 exerts an excellent anti-HSV-2 effect in VK2/E6E7 cells,and it inhibits caspase-1-dependent pyroptosis induced by HSV-2 infection.These data enrich our understanding of the pathologic basis of HSV-2 infection and provide experimental evidence for the anti-HSV-2 activity of JZ-1.

敲减单纯疱疹病毒Ⅱ型(HSV-2)UL30蛋白表达可抑制HSV-2复制

按照shRNA(small hairpin RNA)设计要求,选择编码单纯疱疹病毒Ⅱ型DNA多聚酶催化亚单位的UL30(unique long 30,UL30)基因序列保守区域,设计、合成并构建表达UL30序列特异性siRNA(short interfering RNA)的质粒载体pUL30.通过磷酸钙转染法将其转染入HEK(human embryonic kidney)293细胞中,用蛋白印迹法检测对HSV-2 UL30蛋白表达的影响,观察受染细胞病变效应(cytopathic effect,CPE),终点滴定法测定细胞上清液中病毒感染滴度(50%tissue culture infective dose,TCID50).结果表明,针对UL30基因的siRNA能有效抑制UL30蛋白表达,同时显著抑制受染细胞的CPE,降低上清液中病毒感染滴度.提示本研究建立的针对UL30基因特异性siRNA能有效阻断HSV-2在HEK293细胞内的复制,UL30基因是一个潜在的抗HSV-2复制的药物靶标.

2013—2014年上海市闵行区婚检人群HSV-2感染情况及影响因素分析

目的了解上海市闵行区婚检人群单纯疱疹病毒2型(herpes simplex virus type 2,HSV-2)感染情况及其影响因素。方法对上海市闵行区2013—2014年的婚检人群进行艾滋病相关知识、性行为情况问卷调查。采集血样检测HIV、HSV-2及梅毒感染情况。结果共调查2 116名婚检对象,共有92人感染HSV-2,感染率为4.35%。其中男性感染率为3.69%,女性感染率为5.01%。多因素Logistic回归分析显示,对于男性婚检人群,文化程度为高中及以下(OR=2.47,95%CI:1.195~5.108),未婚妻为HSV-2阳性(OR=9.29,95%CI:4.279~20.164)者更容易感染HSV-2。对于女性婚检人群,年龄≥25岁(OR=9.29,95%CI:4.279~20.164),非上海市户籍(OR=2.19,95%CI:1.091~4.378),文化程度为高中及以下(OR=3.37,95%CI:1.721~6.596),从不使用安全套(OR=3.45,95%CI:1.265~9.392),未婚夫为HSV-2阳性(OR=8.46,95%CI:3.700~19.351)者更容易感染HSV-2。结论上海市闵行区婚检人群的HSV-2阳性率较低,然而安全套使用率低导致未婚夫妻中任何一方感染HSV-2就会增加另一方的感染风险,提示需进一步提高未婚夫妻安全套使用。

细胞MEK1/2蛋白及其相关通路在单纯疱疹病毒Ⅱ型(HSV-2)复制中的作用

基于细胞Raf/MEK/ERK信号通路与病毒复制的关系,应用Western印迹检测p-ERK1/2蛋白的表达、用终点滴定法测定病毒增殖量(TCID50),以及观察感染细胞的细胞病变效应(CPE)等,揭示单纯疱疹病毒Ⅱ型(HSV-2)复制与ERK通路的关系.结果表明,HSV-2的复制可引起细胞ERK通路的活化;用U0126预先抑制ERK通路的活化,或用特异性siRNA敲减MEK1/2基因的表达可显著地抑制病毒复制.提示ERK信号通路以及MEK1/2蛋白对HSV-2的复制具有重要的作用.该研究对进一步阐明细胞ERK通路各激酶蛋白在病毒复制中的作用机制、寻找抗病毒作用靶标等奠定了良好的基础.

黄芪总多糖抗HSV-2的实验研究

目的 :研究黄芪的抗病毒作用。方法 :以阿昔洛韦 (ACV)为阳性对照 ,采用对病毒所致细胞病变的抑制及空斑减数实验 ,观察黄芪总多糖抗HSV 2 333株药效。结果 :在Hep 2细胞系统中 ,ACV对HSV 2 333株直接杀灭、感染阻断、增殖抑制的ED50 分别为 16 .4 5 ,18.6 2 ,10 .85μg/ml;黄芪总多糖的相应数值分别为 6 .0 4 ,5 .4 3,7.5 0 μg/ml。结论 :黄芪总多糖对HSV 2 333株的治疗指数为ACV的 3.7,2 .7,3.3倍 ,值得开发利用。

大玉竹低聚糖硫酸酯抗HSV-2病毒活性的研究

从传统中药大玉竹中提取低聚糖Poos ,用吡啶 氯磺酸法制备了它的硫酸酯衍生物S Poos.产物经红外鉴定 ,证实Poos硫酸酯化后羟基连上了硫酸基 ,硫含量为 8.47% ,取代度 (Ds)为 0 .6 .体外实验研究了Poos、S Poos对非洲绿猴肾细胞 (Vero)的细胞毒性和抗单纯疱疹病毒 2型 (HSV 2 )的活性 .结果表明 ,Poos和S Poos都无细胞毒性 .Poos本身无抗病毒活性 ,对HSV 2引起的细胞病变和空斑形成都无抑制作用 ;经硫酸酯衍生后的S Poos获得抗病毒活性 ,12 5～ 2 0 0 0 μg/mL的S Poos能很好地抑制HSV 2引起的细胞病变 ,2 0 0 μg/mL的S Poos能完全抑制病毒空斑形成 .图 4表 2参

GDNF及HSV-GDNF对坐骨神经损伤大鼠脊髓运动神经元Bcl-2表达的影响

目的 观察胶质细胞源性神经营养因子 (GDNF)及单纯疱疹病毒 (HSV)载体介导的 GDNF(HSV-GDNF)对坐骨神经损伤大鼠脊髓运动神经元 Bcl- 2表达的影响。 方法 分别取坐骨神经损伤后 4d、7d和 14d大鼠(分成对照组、GDNF组和 HSV- GDNF组 )的腰段脊髓 (L4～ 6 ) ,行石蜡包埋、切片 ;用抗 Bcl- 2抗血清进行免疫组织化学染色 ,观察 Bcl- 2免疫反应 (Bcl- 2 - IR)神经元数目 ,并在图像分析仪上对 Bcl- 2 - IR阳性神经元作光密度的色谱分析。 结果 1.坐骨神经损伤后 4d、7d时 ,GDNF组和 HSV- GDNF组损伤侧脊髓运动神经元 Bcl- 2 - IR阳性神经元的数量和平均光密度均明显高于对照组损伤侧。2 .坐骨神经损伤后 14d时 ,对照组、GDNF组和 HSV- GDNF组损伤侧脊髓运动神经元对 Bcl- 2的表达已无明显差别。 结论 GDNF与 HSV- GDNF能够增强坐骨神经损伤大鼠脊髓运动神经元 Bcl- 2的表达 ,减少神经元的退化死亡。

HSV-2 LAT过表达vero细胞中microRNA的表达谱变化

目的分析过表达疱疹病毒Ⅱ型(HSV-2)潜伏相关转录子LAT后vero细胞microRNA表达谱的表达变化。方法通过化学合成的方法获得LAT基因的全长序列。构建HSV-2 LAT逆转录病毒表达载体pRetroQ-AcGFP1-C1,包装获得HSV-2 LAT基因过表达的逆转录病毒。利用microRNA芯片技术,分析感染逆转录病毒HSV-2 LAT后vero细胞microRNA表达谱的变化,得到因LAT基因过表达而产生变化的microRNA。结果通过microRNA芯片分析,逆转录病毒HSV-2 LAT感染vero细胞后,可引起hsa-miR-23a*、kshv-miR-K12-3、hsa-miR-943、hsa-miR-634、hsa-miR-1270 5种microRNA2倍以上上调;使hsa-miR-181a-2*、hsa-miR-450b-5p、hsa-miR-31、hsa-miR-24、kshv-miR-K12-12*5种microRNA2倍以上下调。结论 LAT基因过表达后可引起vero细胞microRNA表达谱的变化。

脂质体转染对HSV-2多表位复合DNA疫苗诱导小鼠特异性免疫应答的影响

目的研究不同免疫方式对HSV-2多表位复合DNA疫苗诱导小鼠免疫应答的影响,探索新型HSV-2DNA疫苗的有效免疫方式。方法利用真核表达质粒pcDNA3.1构建HSV-2糖蛋白gD,gB,gC和早期表达蛋白ICP 27的多表位复合DNA疫苗HV-pcDNA3.1。C57/BL6小鼠分为脂质体包裹pcDNA3.1空载体质粒对照组、脂质体包裹HV-pcDNA3.1质粒和裸质粒HV-pcDNA3.1肌肉注射免疫三组。ELISA检测小鼠血清HSV-2特异性IgG,IL-2和IFN-γ,乳酸脱氢酶法检测杀伤性T淋巴细胞(CTL)活性。结果与裸质粒免疫组相比,脂质体包裹HV-pcDNA3.1免疫组小鼠血清中HSV-2特异性IgG和IFN-γ表达明显增加,CTL活性增强。结论脂质体包裹质粒比裸质粒肌肉注射方式免疫小鼠能显著提高HSV-2多表位复合DNA疫苗的免疫活性。

HSV-2多功能蛋白ICP27真核表达载体构建及其在Vero细胞中的表达

目的构建单纯疱疹病毒2型(HSV-2)多功能蛋白感染细胞多肽27(ICP27)真核表达载体pCDNA3.0-ICP27,并检测其在非洲绿猴肾细胞(Vero)中的表达。方法提取病毒株HSV-2333 DNA,用高保真DNA聚合酶对多功能蛋白ICP27基因进行高保真扩增,用双酶切连接至真核表达载体pCDNA3.0中。pCDNA3.0-ICP27经双酶切、测序验证,并通过脂质体介导质粒瞬时转染Vero细胞,经RT-PCR和Western blot检测ICP27蛋白的表达。结果 pCDNA3.0-ICP27经双酶切可切出目的片段,测序结果经比对,与基因库中的序列完全一致。转染后经RT-PCR和Western blot检测,证实转染重组质粒组有ICP27蛋白表达,而转染空质粒组及未转染组没有检测到ICP27的表达。结论成功构建了HSV-2多功能蛋白ICP27真核表达载体pCDNA3.0-ICP27,并能在Vero细胞中表达。

参芪止疱颗粒抗HSV-2的体外实验研究

目的:探讨参芪止疱颗粒体外抗HSV-2的作用。方法:利用HFF感染HSV-2,用参芪止疱颗粒予以干预,以ACV做对照药,采用CPE法和MTT法进行实验。结果:实验发现HSV-2的TCID50为104;参芪止疱颗粒对HFF的CC50值大于10mg/ml,表明其对HFF的毒性作用小;在药物直接抗病毒复制实验中,参芪止疱颗粒对感染细胞EC50为0.30mg/ml,TI>36表明其对HSV-2感染HFF具有一定保护作用;在HSV-2感染HFF的治疗实验中,参芪止疱颗粒EC50值为0.60mg/ml,TI>25,提示其对病毒感染后复制有一定的抑制作用;其对HSV-2复制的抑制作用时相主要在感染后0h、2h、4h。但是,其对HSV-2感染细胞无预防作用。结论:参芪止疱颗粒在体外试验中具有较好的抗HSV-2的作用,值得临床进一步推广。

PCR检测生殖器疱疹患者HSV-2

目的：用聚合酶链反应（ｐｏｌｙｍ ｅｒａｓｅｃｈａｉｎ ｒｅａｃｔｉｏｎ， Ｐ Ｃ Ｒ）检测生殖器疱疹患者单纯疱疹病毒（ｈｅｒｐｅｓｓｉｍ ｐｌｅｘ ｖｉｒｕｓ ２， Ｈ Ｓ Ｖ２）。方法：对１０１ 例生殖器疱疹和糜烂患者及２０ 例对照组用 Ｐ Ｃ Ｒ法检测 Ｈ Ｓ Ｖ１、 Ｈ Ｓ Ｖ２。结果： Ｈ Ｓ Ｖ２ 检出阳性率占 ６０４％ （６１／１０１）， Ｈ Ｓ Ｖ２ 和 Ｈ Ｓ Ｖ１ 双重感染占４％ （４／１０１）。对照组均为阴性，并且年龄轻者感染阳性率高于年龄长者。结论： Ｐ Ｃ Ｒ 具有操作较易、快速、敏感的特点，为临床对生殖疱疹的诊断和鉴别诊断提供了理想的新方法。