Herpes simplex virus type 1 in peptic ulcer disease: An inverse association with Helicobacter pylori

AIM： To assess the frequency of herpes simplex virus type I in upper gastrointestinal tract ulcers and normal mucosa with the modern and better assays and also with a larger number of well characterized patients and controls and its relationship to Helicobacter pylori（H pylori）. METHODS： Biopsy specimens from 90 patients （34 with gastric ulcer of the prepyloric area and 56 with duodenal ulcer） were evaluated. Biopsies from 50 patients with endoscopically healthy mucosa were considered as the control group. The method used to identify herpes simplex virus-1 （HSV-1） was polymerase chain reaction. Hpylori was detected by the CLO-test and by histological method. RESULTS： Herpes simplex virus-1 was detected in 28 of 90 patients with peptic ulcer （31%） Ⅲ of 34 patients with gastric ulcer （32.4%） and 17 of 56 with duodenal ulcer （30.4%）1 exclusively close to the ulcerous lesion. All control group samples were negative for HSV-1. The likelihood of Hpylori negativity among peptic ulcer patients was significantly higher in HSV-1 positive cases than in HSV-1 negative cases （P = 0.009）. Gastric ulcer patients with HSV-1 positivity were strongly associated with an increased possibility of Helicobacter pylori negativity compared to duodenal ulcer patients （P = 0.010）. CONCLUSION： HSV-1 is frequent in upper gastrointestinal tract ulcers but not in normal gastric andduodenal mucosa. There is an inverse association between HSV-1 and Hpylori infection.

Preliminary study on Herpes simplex virus type 1 infection of human oral epithelial cell in vitro

Objective： To explore the functions and mechanisms of herpes simplex virus type I（HSV-1） while infecting human oral epithelial cells in vitro（being similar to the infection in vivo）. Methods：An abundance of HSV-1 strains amplified in Vero cells were used to infect human oral epithelial cells. The culture supernatant was collected to infect Vero cells again. Morphology of HSV-1 was identified by inverted microscope and transmission electron microscope. Nucleic acid of the virus was detected by PCR. Results：The infected human oral epithelial cells didn＇ t display an obvious cytopathic effect（CPE） under inverted microscope（while Vero cells which were infected by the culture supernatant showed typical（CPE）. The virus particles were not observed in the cytoplasm nor in nucleus of human oral epithelial cells, however under transmission electron microscope in the cytoplasm of Vero cells, the nucleic acid of HSV-1 could be detected in infected human oral epithelial cells, by PCR. Conclusion-HSV-1 can successfully infect human oral epithelial cells. This model may provide a useful approach for studying the pathogenesis of herpes virus-associated periodontal disease.

Expression of Cytokines IL-2, IL-10 and TNF-α in Mice with Herpes Simplex Viral Encephalitis

The expression of the cytokines IL-2, IL-10, TNF-α and their roles in mice with herpes simplex viral encephalitis （HSE） were studied. By using semiquantitative reverse transcription polymerase chain reaction （RT-PCR）, the expressions of IL-2, IL-10 and TNF-α mRNA in control group, HSE group and acyclovir （ACV）-treated group were detected and the pathological changes of brain were observed. It was found that after HSV1 infection, the cerebral lesions of haemorrhage and necrosis in mice were observed under the microscopy, and the levels of IL-2, IL-10 and TNF-α were increased remarkably. After treatment with ACV after HSV1 infection, the cerebral lesions in mice were improved, the level of IL-2 maintained stable, IL-10 was increased consistently, and TNF-α was decreased significantly as compared with those in HSE group. In acute HSE, many cytokines are upregulated, including IL-2, IL-10 and TNF-α to eliminate virus and TH1 type response is dominant. In convalescence, there is a shift in the cytokine expression profile from TH1 profile to TH2 profile and the shift can inhibit the overexpression of immune response in animals. ACV has remarkable effects in the treatment of HSE.

Detection of Varicella Zoster Virus DNA within Lesions and Healed Skin Lesions of Herpes Zoster by PCR

Varicella zoster virus(VZV) DNA in blister lesions and skin biopsies obtained from healed skin lesions in 16 patients with herpes zoster was detected using polymerase chain reaction. A 385 bp VZV DNA fragment was found in all the blister lesions and in two of six biopsies from the skin lesions healed within two months by PCR. No VZV DNA was found in the skin lesions more than two months after healing in 10 cases of herpes zoster. VZV DNA may be detected at the sites of resolved herpes zoster lesions within short duration.

Detection of herpes simplex virus type 1 in rheumatic valvular tissue

Background Rheumatic heart disease (RHD) is the most important sequela of rheumatic fever (RF): evidence that streptococcal infection is aetiological is prominent, but sometimes contradictory. Acute HSV-1 infection in mouse leads to carditis and valvulitis whereas recurrent infection results in inflammatory granulomatous lesions that resemble Aschoff bodies. Cells containing HSV-1 inclusions or virus infected giant cells appear similar to Anitschkow cells or Aschoff cells respectively. We hypothesized that HSV-1 infection also may be involved in RHD. Methods Formalin-fixed, paraffin-embedded valvular tissue samples from 32 patients with RHD were investigated for evidence of HSV-1 infection. HSV-1 antigen was detected by immunohistochemistry, using HSV-1-specific monoclonal and polyclonal antibodies. HSV-1 glycoprotein D gene sequences were amplified by nPCR, using β-globin gene amplification in the same samples as internal control. Valvular tissue from 5 cases of sudden death and 3 cases died of neisseria meningitis without a history of valvular disease was used for comparison. HSV-1-infected lung tissue was used as positive control. Results HSV-1 antigens were detected in valvular tissues from 21 of 32 (65.6%) patients. Fifteen of these 21 (46.9% of cases), but no antigen-negative sample, were positive also for HSV DNA. Nucleotide sequence of PCR products was homologous to the targeted region of the HSV-1 glycoprotein D gene. HSV-1 antigen was present also in one case of sudden death but viral DNA was not found in any tissue sample from the comparison group. Results from reagent and positive controls were as anticipated.Conclusions This is the first study to show the presence of HSV-1 antigen and genomic DNA in valvular tissues from patients with RHD and provides evidence for an association of HSV-1 infection with some cases of rheumatic valvular disease.

生殖器疱疹病毒抗原ELISA与PCR检测结果的对比研究

目的:研究对比酶联免疫吸附法(ELISA法)及聚合酶链反应法(PCR法)在生殖器疱疹病毒抗原检测中的应用价值。方法:随机选取2017年1月至2022年10月在临沂市皮肤病医院进行诊治的疑似生殖器疱疹患者87例,采集患者标本并分别应用ELISA法及PCR法进行单纯疱疹病毒抗原检测。以病毒培养法检测结果作为金标准,分析ELISA法及PCR法在生殖器疱疹病毒抗原检测中的应用效果。结果:两种检测方法对HSV-1感染、HSV-2感染、混合感染的检出率以及总阳性检出率的差异均无统计学意义(P>0.05)。以病毒培养法检测结果为金标准,ELISA法检测与PCR法检测诊断生殖器疱疹灵敏度、准确度、特异度、阳性预测值、阴性预测值的差异均无统计学意义(P>0.05)。结论:ELISA法及PCR法在生殖器疱疹病毒抗原检测中的应用价值均较高,但是ELISA法具有经济实用、操作简单等特点,更加适合基层医院推广和应用。

男性不育患者生精细胞HCMV、HSV感染检测及形态学研究

目的:探讨男性不育患者精液中生精细胞人类巨细胞病毒(HCMV)、单纯疱疹病毒Ⅱ型(HSV-Ⅱ)感染状况及其形态学特征。方法:收集83例精液检查中发现较多生精细胞男性不育患者精液,洗涤收集细胞后提取DNA,用PCR方法进行HCMV、HSV-Ⅱ筛查,阳性者精液细胞涂片用免疫细胞化学法(ICC)做相应的病毒标记,并另行细胞学染色作形态学观察。结果:83例精液样本PCR检测HCMV阳性8例,HSV-Ⅱ阳性4例,未发现2种病毒同时阳性病例。8例HCMV阳性病例ICC标记生精细胞HCMV晚期抗原均见阳性表达,HCMV早期抗原均为阴性表达;4例HSV-Ⅱ阳性病例ICC标记生精细胞3例阳性表达,1例弱阳性。12例病毒阳性病例均发现较多未成熟生精细胞,并有不同程度的核染色质固缩、出现空泡、核膜破损、核崩解、凋亡小体等凋亡现象,但未能找到病毒感染的特异性形态学改变(如病毒包涵体)。病毒感染阳性组精子密度明显低于阴性组(P<0.05)。结论:生精细胞HCMV、HSV-Ⅱ感染时可出现不同程度的病理性损害,影响生精功能,感染的生精细胞形态学表现为出现凋亡现象等病理性改变;不育男性患者精液中出现病理性生精细胞,其生精细胞HCMV感染率可能较高。

单纯疱疹病毒1型糖蛋白D核酸疫苗的构建及初步免疫观察

目的 构建用于防治单纯疱疹的核酸疫苗并观察其免疫效果。方法 用PCR反应 ,从HSV 1F株基因组DNA中扩增出 gD蛋白的全部编码序列 ,将其插入 pcDNA 3 1 (+)的PCMV下游 ,构建HSVgD核酸疫苗 ,并用酶切分析和测序鉴定 ;通过中和试验、ELISA方法和攻击试验检测用 pLy D三次肌肉接种小鼠的免疫效果。结果 经鉴定证实了HSV gD核酸疫苗 pLy D的构建 ;实验小鼠产生了对HSV 1特异性的抗体 (抗体滴度 :ELISA法 1∶2 0 3,中和试验法 1∶37) ,并经受了HSV 1病毒的攻击 (存活率 :70 % )。结论 成功构建出了HSV gD核酸疫苗pLy D ,用其接种小鼠可以诱导产生特异性免疫反应 ,并具有良好的保护作用。

聚合酶链反应诊断单纯疱疹病毒性脑炎

用聚合酶链反应（ＰＣＲ）扩增患者脑脊液（ＣｈＦ）中病毒特异性ＤＮＡ可早期快速诊断单纯疱疹病毒性脑炎（ＨＳＥ）。１９例临床确诊的病毒性脑炎患者，经ＰＣＲ在ＣＳＦ中检出单纯疱疹病毒（ＨＳＶ）１３例，全部阳性标本均经分子杂交证实为ＨＳＶ－ＤＮＡ，而１４例其他神经疾病（ＯＮＤ）对照组均为阴性，显示了这一方法的特异性。其中７例病毒性脑炎ＣＳＦ标本分别用ＰＣＲ分子杂交和病毒分离等三种方法检测ＨＳＶ；显示ＰＣＲ最为敏感。表明ＰＣＲ技术的广泛应用将提高ＨＳＥ的早期诊断水平，指导临床正确治疗。

应用原位聚合酶链反应检测淋病患者HSV-Ⅱ感染情况的报告

为了解淋病患者ＨＳＶⅡ的感染情况，应用原位聚合酶链反应（ＩＳＰＣＲ）和ＰＣＲ技术对５８例淋病患者进行ＨＳＶⅡ检测。结果两种方法ＨＳＶⅡＤＮＡ阳性检出率均为５３．４５％（３１／５８）。ＩＳＰＣＲ显示，１１例有皮损者中，９例阳性信号存在于上皮细胞核及胞浆，既往有疱疹皮损者６例，阳性信号均存在于细胞核，４１例无明显皮损者，１６例阳性，其中１２例阳性信号在细胞核，４例在胞核及胞浆。结果提示，淋病患者合并有高的ＨＳＶⅡ感染率。应用ＩＳＰＣＲ不仅可以敏感特异地检测ＨＳＶⅡ，而且可以定位。

自然流产孕妇巨细胞病毒与单纯疱疹病毒感染的研究

目的:探讨自然流产孕妇中巨细胞病毒与单纯疱疹病毒感染的状况。方法:留取132例自然流产孕妇及113例因计划外妊娠行人工流产者(对照组)的绒毛组织,用荧光定量多聚酶链反应技术检测绒毛组织标本中巨细胞病毒和单纯疱疹病毒的基因数量。结果:自然流产组孕妇中巨细胞病毒阳性率为16.67％(22/132),对照组阳性率为1.91％(2/113),差异有显著性(P<0.005)。自然流产组孕妇单纯疱疹病毒阳性率为17.42％(23/132),对照组阳性率为2.65％(3/113),差异有显著性(P<0.005)。两者皆为阳性者自然流产组孕妇有12例,占9.09％,对照组均为阴性。治疗后复查巨细胞病毒和单纯疱疹病毒阴性的妇女再次妊娠成功。结论:巨细胞病毒和单纯疱疹病毒均可导致孕妇发生自然流产,且巨细胞病毒及单纯疱疹病毒易合并存在,因此,对自然流产孕妇应同时检测巨细胞病毒及单纯疱疹病毒,针对病因进行治疗,提高下一次妊娠成功率。

细胞培养与PCR法检测生殖器疱疹病毒的对比研究

目的：比较不同方法检测生殖器疱疹病毒感染的效率。方法：采用病毒培养和PCR法检测疑为生殖器疱疹病毒感染者标本60例，并用PCR作病毒分型。结果：根据病史及临床表现确诊的生殖器疱疹患者标本60例中，病毒培养法阳性36例，阳性牢60％（36／60）；PCR检测单纯疱疹病毒（HSV）阳性45例，阳性率75％（45／60），和病毒培养相比，差异非常显著（χ^2=26．76，P〈0．01）；PCR分型结果显示阳性标本均为单纯疱疹病毒Ⅱ型（HSV-2）。水疱和脓疱标本的病毒培养和PCR检测阳性率均较高（80．0％～93．3％），糜烂、结痂、斑丘疹标本检测中PCR阳性率（20．0％～66．7％）高于病毒培养（0～33．3％）。结论：对疑为生殖器疱疹患者作病原学诊断，采集水疱、脓疱标本进行病毒分离或PCR检测较佳。

抗原捕获聚合酶链反应分型检测妇女生殖器单纯疱疹病毒

目的 : 建立直接分型检测妇女生殖器单纯疱疹病毒 (HSV)的抗原捕获聚合酶链反应 (AC -PCR)。方法 : 用抗HSV型共同性糖蛋白单克隆抗体 ,包被聚苯乙烯离心管 ,捕获HSV ,同时加入 3个引物 :HSV - 1 HSV - 2型共同性上游引物及HSV - 1和HSV - 2型特异性下游引物 ,进行PCR扩增。结果 :HSV - 1和HSV - 2标准病毒株均分别扩增出与设计大小相符的 4 77bp和 399bpDNA条带。AC -PCR可检测到 10PFUHSV - 1和 1PFUHSV - 2。用AC -PCR检测了 36 5份妇女生殖器拭子标本 ,阳性 10 1例(2 7.7% ) ,2 3例为HSV - 1(占 2 2 .8% ) ,78例为HSV - 2 (占 77.2 % ) ;其中 112份标本同时用AC -PCR和分离培养法检测 ,AC -PCR的阳性率为 2 6 .8% (30 112 ) ,分离培养法的阳性率为 2 0 .5 % (2 3 112 ) ,两者差异有显著性 (χ2 =4 .5 ,P <0 .0 5 )。结论 : AC -PCR是特异、敏感。

低体质量新生儿和新生儿肺炎常见病原体筛查

目的探讨出生缺陷新生儿中低体质量和肺炎新生儿人巨细胞病毒(HCMV)、单纯疱疹病毒Ⅰ型(HSV-Ⅰ)、HSV-Ⅱ、弓形虫(TOX)、乙肝病毒(HBV)5种病原微生物感染情况,分析巢式聚合酶链反应法检测新生儿病原体感染的临床应用价值。方法选取低体质量新生儿46例和肺炎新生儿66例,每例抽取外周静脉血1mL。经曲酚-氯仿-异戊醇-蛋白消化法,提取外周血血清中的DNA,通过二对引物,一对扩增较大DNA片段的外引物和一对在扩增产物中再扩增小片段的内引物,采用巢式PCR法,分别针对HCMV、HSV-Ⅰ、HSV-Ⅱ、TOX、HBV病毒DNA高度保守区设计引物并扩增其病毒DNA,检测这5种病毒DNA在低体质量和肺炎新生儿中感染阳性率,筛查这些病毒在出生缺陷新生儿中的感染状况。采用SPSS10.0软件分析5种病原体感染率之间的关系。结果低出生体质量新生儿46例中,5种病原体检出率:HCMV为91.3%、HSV-Ⅰ为8.7%、HSV-Ⅱ为15.2%、TOX为8.7%、HBV为15.2%;肺炎新生儿66例中,5种病原体检出率:HCMV为83.3%、HSV-Ⅰ为6.1%、HSV-Ⅱ为16.7%、TOX为6.1%、HBV为7.6%。HCMV感染率在低体质量儿和肺炎患儿中均高于其他4种病原体,且5种病原体感染率有统计学意义(Pa=0)。结论对低体质量和肺炎新生儿病原体感染进行筛查十分必要,且对新生儿感染性疾病的早期诊断和预防有益。

荧光定量聚合酶链反应对生殖器疱疹病毒感染的检测

目的探讨荧光定量聚合酶链反应(FQ-PCR)在诊断生殖器疱疹病毒感染中的应用。方法本研究共分两组,检测组即就诊的疑似生殖器疱疹患者347例,对照组12例。分别用FQ-PCR方法检测两组送检标本中的单纯疱疹病毒(HSV)DNA。结果347例疑似生殖器疱疹患者送检标本中,HSV DNA阳性139例,阳性率为40.1%(139/347),其中阳性标本中有皮损组织液75例、男性尿道拭子31例、女性宫颈分泌物33例,各类标本的阳性率依次为91.5%(75/82)、21.1%(31/147)、28.0%(33/118)。HSV DNA阳性人群中性别差异无统计学意义(P>0.05,χ2检验)。12例对照标本中没有检出HSV DNA。结论分泌物中检出的HSV DNA能直观地反映患者当前病毒感染状况,在有皮损组织的患者中,HSV DNA的检出率更高,FQ-PCR能准确、快速地对生殖器疱疹病毒感染做出诊断。

多重聚合酶链反应快速诊断HSK和真菌性角膜炎的研究

目的:探讨多重聚合酶链反应(multiplexPCR,MPCR)技术快速诊断单纯疱疹病毒性角膜炎(HSK)和真菌性角膜炎的价值。方法:建立单纯疱疹病毒(HSV)和致病性真菌菌株的MPCR检测方法,检测49例患者54眼角膜刮片或泪液标本,对怀疑为真菌和混合感染的与涂片镜检和真菌培养比较。结果:MPCR5h可检测出标本中微量HSV和真菌,54份标本MPCR检测阳性43份(80%),其中怀疑有真菌感染的25份标本中17份真菌检测阳性(68%),阳性率明显高于真菌培养(χ2=11.57,P<0.005)和涂片镜检(χ2=13.33,P<0.005)。结论:MPCR速度快、敏感性和特异性高,有助于HSK和真菌性角膜炎的快速明确诊断。

聚合酶链反应检测宫颈糜烂患者单纯疱疹病毒感染

目的 :探讨宫颈糜烂患者单纯疱疹病毒 (HSV)感染情况。方法 :用聚合酶链反应检测宫颈糜烂患者和正常对照组单纯疱疹病毒感染情况。结果 :10 2例宫颈糜烂患者中 ,HSV- 1和 HSV- 2阳性率分别是 4 .9%和 30 .4 % ,正常对照组中 ,HSV- 1和 HSV- 2阳性率分别为 2 .7%和 12 .0 %。结论 :HSV感染与宫颈糜烂关系密切 ,且以 HSV- 2感染为主。

我国单纯疱疹病毒Ⅰ型168株糖蛋白D基因的克隆及其在痘苗病毒天坛株中的表达

将我国单纯疮疹病毒Ⅰ型１６８株基因组ＤＮＡ中扩增出的糖蛋白Ｄ基因，插入痘苗病毒ｐ７．５启动子下游，使其在痘苗病毒天坛株表达。免疫荧光分析表明，产生的重组病毒糖蛋白Ｄ能被运到被重组病毒感染的１４３细胞表面表达，表达的产物经Ｗｅｓｔｅｍｂｌｏｔ鉴定为分子量约５０ｋＤ的多肽。Ｓｏｕｔｈｅｍｂｌｏｔ证明重组病毒基因组中整合有ＨＳＶ－１１６８株糖蛋白基因片段，重组病毒免疫家兔后，产生了高滴度的ＨＳＶ特异性中和抗体。

表达HSV－2 gD基因的重组痘苗病毒保护小鼠对抗致死量HSV病霉攻击

利用ＰＣＲ方法对单纯疱疹病毒Ⅱ型糖蛋白Ｄ（ＨＳＶ－２ｇＤ）基因进行了修饰，在其５＇端删去约５００ｂｐ的非编码区，仅保留ＡＴＧ上游７个ｂｐ。将修饰后的ＨＳＶ－２ｇＤ基因插入到带有痘苗病毒天坛株ＴＫ基因区段的痘苗表达质粒ｐＪＳＡ１１７５，置于痘苗病毒Ｐ７．５ｋ早／晚期启动子控制下。将此重组质粒用脂质体Ｌｉｐｏｆｅｃｔｉｎ方法转染已受野型ＴＫ￣＋痘苗病毒天坛株感染的ＴＫ￣－１４３细胞，通过同源重组机制和标志基因ＬａｃＺ产物的蓝斑显色作用，以及ＢｕｄＲ试剂对ＴＫ表型的选择压力，筛选出整合有ＨＳＶ－２ｇＤ基因的重组痘苗病毒。Ｓｏｕｔｈｅｍ杂交表明，ＨＳＶ－２ｇＤ基因已正确地插入痘苗病毒ＴＫ基因区内；间接免疫荧光检测显示，ＨＳＶ－２ｇＤ蛋白已得到有效表达，且主要分布于细胞膜。重组病毒免疫家兔可产生明显的抗ＨＳＶ－２ｇＤ中和抗体。用重组病毒免疫小鼠，３周后可使９４％（１７／１８）的小鼠对抗ＨＳＶ－２的致死量攻击，表明重组病毒具有明显的免疫保护作用。

聚合酶链反应（PCR）对单纯疱疹病毒性脑炎的临床诊断价值

应用聚合酶链反应（ＰＣＲ）检测技术对１１８例颅内感染性疾病患者及３７例无神神经系统疾病患者脑脊液（ＣＳＦ）中的单纯疱疹病毒ＤＮＡ（ＨＳＶ－ＤＮＡ）进行了检测及分型。结果提示：“散发性脑炎”组的阳性率为３８．４６％（２０／５２），细菌、真菌性脑膜炎、其它病毒性脑炎组以及无神经系统疾病组均为阴性。作者认为：①本检测是目前单纯疹病毒性脑炎（ＨＳＥ）较为简便而准确的早期诊断方法之一；②ＨＳＶ分型检测，对病原诊断更具有全面性；③两型单纯疱疹病毒均可引起ＨＳＥ。