HIV-1感染者免疫活化对宿主限制因子SAMHD1表达和HIV-1 DNA水平的影响

目的研究HIV-1感染者CD4;T细胞免疫活化与外周血宿主限制因子SAMHD1表达水平和HIV-1 DNA的关系。方法选取未接受抗病毒治疗的HIV-1感染者57例,接受抗病毒治疗且病毒载量低于检测限的HIV-1感染者62例,健康对照48例。分离外周血单个核细胞(PBMC)和CD4;T细胞,提取总RNA,RT-PCR法检测SAMHD1 mRNA表达水平及血浆HIV-1 RNA水平,流式细胞术检测CD4;T和CD8;T细胞数量及CD4;T细胞免疫活化水平,ELISA检测血浆干扰素α水平,PCR法检测外周血HIV-1 DNA水平。结果未接受抗病毒治疗的HIV-1感染者CD4;T细胞免疫活化水平最高,抗病毒治疗组显著降低,但仍高于健康对照组(P <0.01)。未接受抗病毒治疗组外周血HIV-1 DNA水平显著高于抗病毒治疗组(P <0.01)。HIV-1感染者PBMCs中SAMHD1 mRNA水平显著高于健康对照组(P <0.01),而CD4;T细胞中SAMHD1 mRNA表达水平显著低于健康对照组(P <0.01)。CD4;T细胞SAMHD1 mRNA表达水平与免疫活化呈负相关,但与HIV-1 DNA水平无相关性。结论 HIV-1感染者CD4;T细胞SAMHD1表达水平降低,与免疫活化水平负相关,但与HIV-1 DNA水平无直接相关。

外周血HIV-1 DNA在艾滋病疗效评估中的应用

目的通过研究HIV感染者HIV-1 DNA与HIV-1 RNA及CD4^(+)T淋巴细胞间的关系,探讨外周血HIV-1 DNA在艾滋病疗效评估中的应用。方法筛选2018年6—9月贵州省贵阳市公共卫生救治中心的HIV感染者80例,采用面对面问卷调查收集患者资料,并采集患者K2EDTA抗凝血,完成CD4^(+)T淋巴细胞、HIV-1 RNA及HIV-1 DNA的检测并得出结果。通过SPSS等软件分析HIV感染者的病毒库水平,以及HIV-1 DNA与HIV临床分期、CD4^(+)T淋巴细计数及HIV-1 RNA的相关性。结果HIV感染者CD4^(+)T淋巴细胞数量越多,HIV-1 RNA含量越低,其全血中HIV-1 DNA的水平越低,差异均有统计学意义(P<0.05)。结论HIV-1 DNA可反映抗逆转录病毒治疗(HAART)期间病毒库水平,提示疾病进展情况,评价治疗效果,可为贵州省艾滋病的治疗提供更精准的监测手段。

滤纸片干血斑用于HIV-1 DNA检测的评价

目的探索滤纸固定艾滋病病毒Ⅰ型核酸(HIV-1 DNA)的稳定性、均一性,评价滤纸片干血斑HIV-1DNA检测方法的敏感性、特异性。方法套式PCR扩增HIV-1的env、gag、pol三区。不同环境条件下保存的滤纸片干血斑,分别在不同的时间段检测;滤纸片干血斑的中心及圆斑的上下左右4个边缘,随机打取5个2.5mm圆片用于检测。采自新疆现场的94份阴性样本和90份阳性样本,分别制成滤纸片干血斑样本和全血样本,比较两者的HIV-1DNA检测结果。结果滤纸片干血斑-20℃或4℃放置1年或室温放置3个月,或在37℃放置两天或冻融2次,实验的敏感性未见下降;37℃放置3天或冻融3次,已经有样本不能检出。滤纸干血斑不同位点随机打取圆片扩增,4个样本中,中点均阳性,但在上点、左点、右点分别出现一份阴性结果。滤纸干血斑法和全血法检测HIV-1前病毒DNA比较,敏感性是96.1%,特异性是98.9%。结论滤纸干血斑在室温条件下运输是可行的,推荐尽量靠近滤纸干血斑的中间位点打取圆片扩增;该方法操作简便、经济、敏感、特异。

滤纸片干血斑HIV-1 DNA检测方法的建立

目的探索用滤纸片作血液样本的载体,建立一种简单、经济、敏感的滤纸片干血斑艾滋病病毒Ⅰ型(HIV-1)DNA检测方法。解决HIV-1感染者全血样本采集、运输和储存过程中存在的实际困难。方法首先用滤纸片FTA卡收集血液制成滤纸片干血斑,处理提取DNA后,针对HIV的env、gag、pol区,设计三对高度保守引物,套式PCR扩增HIV-1 DNA。进一步用HIV-1质粒DNA检测该方法的最低检测限。结果摸索出扩增滤纸片干血斑HIV-1 DNA的最佳扩增条件;滤纸片干血斑样本pol区最低检测限是6拷贝/μl,env区8拷贝/μl,gag区10拷贝/μl。结论可以用滤纸片FTA卡收集HIV-1感染者的血液,制成滤纸片干血斑后检测HIV-1 DNA。该方法操作简便、经济、敏感,建议作为HIV-1抗体检测的辅助诊断方法。

Investigation of the interaction between HIV-1 DNA and cyclic peptides by electrospray ionization mass spectrometry

The interaction between HIV-1 DNA and five cyclic peptides （CP1-CP5） was investigated using electrospray ionization mass spectrometry （ESI-MS）. It revealed that CP1 [c（Ala-Tyr-Leu-Ala-Gly）] and CP4 [c（Pro-D-Tyr-Leu-D-Ala-Gly）] have the higher binding affinity with the duplex DNA among the five cyclic peptides.

扩增潜伏HIV-1 DNA序列实验方法的优化

目的对PCR扩增潜伏HIV-1DNA序列的实验方法进行优化。方法收集30例经高效抗逆转录病毒治疗（HAART）6~12个月的HIV-1感染者抗凝血标本,分别从外周血单个核细胞（PBMC）和高度纯化的CD4＋T细胞提取基因组DNA,巢式PCR扩增HIV-1env的C2-V5区,电泳检测扩增产物并进行DNA序列测定。结果同一患者PBMC纯化CD4＋T细胞标本扩增HIV-1env基因C2-V5区的效率（93.3%）明显高于直接从PBMC标本扩增该目的片段的效率（10.0%）。结论 PBMC纯化CD4＋T细胞后,再提取基因组DNA进行巢式PCR扩增,可提高扩增潜伏HIV-1DNA序列的效率。

疟疾感染对HIV-1 DNA疫苗免疫效果的影响

目的探讨小鼠感染疟疾后是否会对艾滋病疫苗的免疫产生影响。方法用HIV-1 DNA疫苗p VAX-gag分别免疫感染过疟疾和未感染过疟疾的Balb/c小鼠,观察不同组小鼠接种p VAX-gag疫苗后,细胞免疫、体液免疫和免疫记忆的变化。结果p VAX1-gag免疫感染过疟疾和未感染过疟疾的Balb/c小鼠,均可诱导出明显的体液免疫和细胞免疫反应;但p VAX1-gag免疫未感染过疟疾的小鼠诱导出的体液免疫反应高于感染过疟疾的小鼠,所获得的抗体滴度是感染过疟疾的小鼠的3倍,未感染过疟疾的小鼠诱导出的细胞免疫反应高于感染过疟疾的小鼠。结论感染疟疾后对艾滋病疫苗的免疫有一定的抑制作用,这为艾滋病疫苗的研发提供了实验依据。

Modulation of cellular and humoral immune responses to anHIV-1 DNA vaccine by interleukin-12 and interleukin-18 DNA immunization

Objective: To investigate the effect of interleukin-12 (IL-12) and interleukin-18 (IL-18)DNA immunization on immune response induced by HIV-1 DNA vaccine and to explore new strategies for therapeutic HIV DNA vaccine. Methods: The recombinant expression vector pCI-neoGAG was constructed by inserting HIV Gag gene into the eukaryotic expression vector pCI-neo. Balb/c mice were immunized with pCI-neoGAG alone or co-immunized with the DNA encoding for IL-12 or IL-18.Anti-HIV antibody and IFN-γ were tested by ELISA,and splenocytes were isolated for detecting antigen-specific lymphoproliferative responses and specific CTL response by MTT assay and LDH assay respectively. Results: The anti-HIV antibody titers of mice co-immunized with pCI-neoGAG and the DNA encoding for IL-12 or IL-18 were lower than that of mice immunized with pCI-neoGAG alone(P<0.01). In contrast, the IFN-γ level of mice co-immunized with pCI-neoGAG and the DNA encoding for IL-12 or IL-18 was higher than that of mice immunized with pCI-neoGAG alone (P<0.01).Furthermore, compared with mice injected with pCI-neoGAG alone, the specific CTL cytotoxity activity and antigen-specific lymphoproliferative responses of mice immunized with pCI-neoGAG and the DNA encoding for IL-12 or IL-18 were significantly enhanced respectively (P<0.01). Conclusion: The DNA encoding for IL-12 or IL-18 together with HIV DNA vaccine may enhance specific Th-1 responses and cellular immune response elicited in mice. Hence, the DNA encoding for IL-12 or IL-18 are promising immune adjuvants for HIV-1 DNA vaccine.

Development of a droplet digital polymerase chain reaction assay for the sensitive detection of total and integrated HIV-1 DNA

Background:Total human immunodeficiency virus(HIV)DNA and integrated HIV DNA are widely used markers of HIV persistence.Droplet digital polymerase chain reaction(ddPCR)can be used for absolute quantification without needing a standard curve.Here,we developed duplex ddPCR assays to detect and quantify total HIV DNA and integrated HIV DNA.Methods:The limit of detection,dynamic ranges,sensitivity,and reproducibility were evaluated by plasmid constructs containing both the HIV long terminal repeat(LTR)and human CD3 gene(for total HIV DNA)and ACH-2 cells(for integrated HIV DNA).Forty-two cases on stable suppressive antiretroviral therapy(ART)were assayed in total HIV DNA and integrated HIV DNA.Correlation coefficient analysis was performed on the data related to DNA copies and cluster of differentiation 4 positive(CD4^(+))T-cell counts,CD8^(+)T-cell counts and CD4/CD8 T-cell ratio,respectively.The assay linear dynamic range and lower limit of detection(LLOD)were also assessed.Results:The assay could detect the presence of HIV-1 copies 100%at concentrations of 6.3 copies/reaction,and the estimated LLOD of the ddPCR assay was 4.4 HIV DNA copies/reaction(95%confidence intervals[CI]:3.6-6.5 copies/reaction)with linearity over a 5-log_(10)-unit range in total HIV DNA assay.For the integrated HIV DNA assay,the LLOD was 8.0 copies/reaction(95%CI:5.8-16.6 copies/reaction)with linearity over a 3-log 10-unit range.Total HIV DNA in CD4^(+)T cells was positively associated with integrated HIV DNA(r=0.76,P<0.0001).Meanwhile,both total HIV DNA and integrated HIV DNA in CD4^(+)T cells were inversely correlated with the ratio of CD4/CD8 but positively correlated with the CD8^(+)T-cell counts.Conclusions:This ddPCR assay can quantify total HIV DNA and integrated HIV DNA efficiently with robustness and sensitivity.It can be readily adapted for measuring HIV DNA with non-B clades,and it could be beneficial for testing in clinical trials.

HIV-1 DNA影响因素及临床价值分析

目的探讨HIV-1 DNA的影响因素及其临床价值。方法选取304例HIV感染/艾滋病患者,分析HIV-1 DNA与CD4^(+)T细胞计数、CD4/CD8、HIV病毒载量、亚型之间的关系,以此探讨HIV-1 DNA的影响因素及临床应用价值。结果不同CD4^(+)T细胞水平组HIV-1 DNA载量不存在统计学差异(Z=1.194,P>0.05)。CD4/CD8≤0.5组HIV-1 DNA载量高于CD4/CD8>0.5组(Z=-2.788,P<0.01)。HIV病毒载量>100拷贝/ml组HIV-1 DNA载量高于≤100拷贝/ml组(Z=-2.953,P<0.01)。确诊时CD4^(+)T细胞计数≤200(细胞/μl)组HIV-1 DNA载量高于CD4^(+)T细胞计数>200(细胞/μl)组(Z=-2.175,P<0.05)。确诊时CD4/CD8≤0.2组患者HIV-1 DNA载量虽高于CD4/CD8介于0.2~0.5之间组,但两组之间比较没有统计学差异(Z=-0.893,P>0.05)。两组HIV-1 DNA载量均高于CD4/CD8≥0.5组(Z=-2.568,Z=-1.960,P<0.05)。确诊时HIV病毒载量>100000拷贝/ml组HIV-1 DNA载量高于HIV病毒载量≤100000拷贝/ml组(Z=-3.520,P<0.001)。CRF01_AE组HIV-1 DNA载量高于非CRF01_AE组,差异存在统计学意义(Z=-2.848,P<0.01)。CD4/CD8为HIV-1 DNA浓度高于500拷贝/ml的保护性因素(OR=0.214(95%CI:0.056~0.822,P<0.05)。结论CD4^(+)T淋巴细胞计数、CD4/CD8、病毒载量及亚型是影响HIV-1 DNA水平的因素,同时HIV-1 DNA可能对于免疫状态评估、疾病进程判断具有辅助作用。

血浆HIV-1 RNA与干血斑HIV-1 DNA基因型耐药检测比较

目的通过对不同病毒载量的同一研究对象同时进行血浆HIV-1 RNA与干血斑HIV-1 DNA的基因型耐药检测并对结果进行比较,探讨HIV-1 DNA用于耐药检测的可行性和用途。方法2021年12月采集云南省、广西壮族自治区及新疆维吾尔自治区接受ART后1年以上的HIV/AIDS患者静脉血5 mL,EDTA抗凝,分离血浆和制备成干血斑样本,分别提取病毒DNA和RNA进行pol区扩增,比较两种方法的扩增效率;并对同时扩增成功的序列利用MEGA7构建系统进化树并分析序列一致性。利用斯坦福大学HIV耐药数据库进行耐药位点分析,比较耐药性结果。结果209例样本中,来自云南82份(39.2%),来自广西壮族自治区69份(33.0%),来自新疆维吾尔自治区58份(27.8%)。105例VL<20拷贝/mL,25例20拷贝/mL≤VL<200拷贝/mL,42例200拷贝/mL≤VL<1000拷贝/mL,37例VL≥1000拷贝/mL。不同病毒载量的样本分类中,使用血浆中HIV-RNA pol区扩增成功率分别为12.4%、28.0%、69.0%、89.2%;使用干血斑中HIV-DNA pol区扩增成功率分别为39.0%、52.0%、59.5%、73.0%;血浆结合干血斑各组的扩增成功率为41.0%、56.0%、76.2%、89.2%。两种耐药检测方法同时扩增成功66例,耐药结果完全一致为98.5%,序列一致性99.7%。其中有58例(58/66,87.9%)配对样本耐药位点完全一致,8例配对样本耐药位点不完全一致。耐药位点不完全一致的配对样本中仅1例导致耐药结果不同,其他主要由混合碱基导致但未对耐药结果产生影响。结论应用干血斑HIV-1 DNA进行基因型耐药检测可以弥补目前血浆HIV-1 RNA耐药检测不足,特别是对病毒载量<1000拷贝/mL的样本,能够提高耐药检测效率。同时二者检测结果基因序列与耐药位点的一致性很好。结合干血斑样本容易制备、保存与运输的优点,提高了在偏远欠发达地区进行耐药监测的可及性。

Evolution of Mother-to-Child HIV-1 Transmission Rate in Mali from 2009 to 2018

Despite enormous efforts to achieve the goal of eliminating mother-to-child transmission of HIV-1, it remains a major challenge for many countries in sub-Saharan Africa, particularly Mali. Our objective is to assess changes in the rate of mother-to-child transmission of HIV-1. We conducted a cross-sectional study between January 1, 2009 to December 31, 2018 (10 years) of early diagnosis activity in newborns and children born to HIV-1-positive mothers at the National Institute for Public Health (INSP). The samples came from health and referral centers in mali. All samples were received at the Laboratory of Molecular Biology at the INSP. Proviral DNA extraction was performed from a blood spot sample with a Roche DNA kit, Cobas AmpliPrep/Cobas TaqMan HIV-1 qualitative Test, V2.0 (Roche Molecular System, Inc, USA) following the company procedures. Molecular diagnosis was performed using the same kits using an algorithm of three identical PCRs. The Epi Info version 7 software was used for data analysis with a significance threshold of 5%. A total of 10,714 samples of infants and children born to HIV-positive mothers were analyzed by PCR. Ninety-six percent of mothers were on ARV prophylaxis (AZT 3TC NVP and AZT NVP) and 60% of newborns received the same ARV prophylaxis. Of these children, 956 tested positive with an overall transmission rate of 8.92%, varying between 7.27% in 2009 and 08.01% in 2018. This rate was relatively low among children receiving prophylaxis at 2.04% and remained high for children who received breastfeeding at 5.62%. However, the transmission rate remains low for those who have benefited from mixed and artificial breastfeeding at 1.58% and 1.27% respectively. A significant proportion of children remained infected by their mothers during pregnancy, childbirth or breastfeeding. This study shows the importance of early diagnosis of HIV in children using molecular technology.

广西钦州市新报告HIV/AIDS抗病毒治疗1年后HIV-1 DNA载量变化分析

目的了解广西钦州市部分新报告HIV/AIDS接受抗病毒治疗1年后HIV-1 DNA载量变化。方法广西钦州市2019年9月至10月新报告感染病例、确证1个月内开始抗病毒治疗者36例,分别于治疗前(基线)和治疗12个月时采集患者外周血,进行HIV pol基因测序、血浆病毒载量、CD4^(+)T淋巴细胞数及HIV-1 DNA载量检测,分析HIV-1 DNA载量的变化。结果调查对象的HIV亚型包括CRF01_AE(55.6%,20/36)、CRF08_BC(33.3%,12/36)和其他(11.1%,4/36);基线病毒载量均大于1000 copies/mL,治疗12个月后91.7%(33/36)的患者病毒载量低于1000 copies/mL,其中30人低于检测限;基线和治疗12个月后CD4^(+)T淋巴细胞数中位数分别为177个/µL和313个/µL(P<0.001);HIV-1 DNA载量中位数分别为3.26 log_(10) copies/10^(6) PBMCs和2.15 log_(10) copies/10^(6) PBMCs(P<0.001)。多因素分析表明低基线HIV-1 DNA载量和非CRF01_AE毒株是治疗12个月后HIV-1 DNA载量降至2 log_(10) copies/10^(6) PBMCs的相关因素。结论抗病毒治疗1年后患者HIV-1 DNA载量下降,基线HIV-1 DNA载量和HIV毒株类型可能与治疗后HIV-1 DNA载量相关。

基线极高HIV-1 RNA水平对初治HIV-1感染者外周血total HIV-1 DNA的影响

目的观察基线HIV-1 RNA>50万copies/mL的HIV-1感染者,在高效抗反转录病毒治疗(highly active antiretroviral therapy,HAART)前后外周血totalHIV-1 DNA的变化。方法从国家十二五科技重大专项课题中选取基线HIV-1 RNA>50万copies/mL且HAART 96周HIV-1 RNA<50 copies/mL的初治HIV-1感染者为试验组,年龄性别相当的基线HIV-1 RNA<50万copies/mL的HIV-1感染者为对照组。检测两组患者基线和HAART 24、48、96周时total HIV-1 DNA水平。结果基线及HAART 96周,试验组total HIV-1 DNA均高于对照组3.48(3.21~3.80)lg copies/106 PBMCsvs 2.90(2.54~3.30)lg copies/106 PBMCs(p<0.001),2.82(2.38~2.96)lgcopies/106 PBMCs vs 2.37(1.99~2.65)lg copies/106 PBMCs(p=0.001)。HAART 24周、48周,试验组detal HIV-1 DNA较对照组高0.67(0.41~1.03)lg copies/106 PBMCs vs 0.39(0.09~0.73)lg copies/106 PBMCs(P<0.001),0.8(0.46~1.16)lg copies/106 PBMCs vs 0.43(0.04~0.63)lg copies/106 PBMCs(P<0.001)。且HAART前后total HIV-1 DNA水平均与基线病载正相关。结论基线极高病载患者HAART 96周内存在较高total HIV DNA水平,建议选择强效HAART方案来有效降低储存库。

The Biochemical Impact by Covalent Shielding of the Anionic Oxygen of the Phosphate Group in DNA and RNA as Methylated Phosphotriester Linkage on the Inhibition of DNA Duplication and on HIV-1 RNA Viral Infectivity Has Been Seriously Overlooked

With the help of model experiments, we are able to offer a detailed proposal for the inhibition of DNA duplication and no inhibition of RNA viral infectivity. As a backbone, we introduced methyl phosphotriester (MPTE). Duplex formation according to the traditional Watson and Crick base-pairing: [(MPTE)n−1 DNA] * DNA and [(MPTE)n−1 DNA] * RNA, where n = number of DNA and RNA bases. However, in the latter case, inhibition is obtained by reduction of the number of MPTE linkages, as is confirmed with model experiments and under biological conditions with micro (mi)RNA substrates. The latter results have recently been published. One or more single MPTEs are disseminated over different places of DNA without neighbour MPTEs (Prof. Wen-Yih Chen and his group, Taiwan).

HIV-1 RNA被有效抑制下T细胞与外周血中HIV-1前病毒DNA

目的:考察HIV-1 RNA被有效抑制下T细胞与外周血中HIV-1前病毒DNA的相关性。方法:对云南地区90例确诊为AIDS,HAART持续治疗时间超过6个月,血浆HIV RNA<50 Copies/ml的患者进行研究,采用Spearmans秩和相关回顾性分析CD4+、CD3+、CD8+、CD4+CD28+、CD4+CD45RA+、CD4+CD45RO+、CD38+、CD8+CD38+T细胞的绝对计数和相对计数与外周血中HIV-1前病毒DNA的相关性,同时考察HIV-1前病毒DNA拷贝数与HAART持续治疗时间的相关性。将90例患者根据HAART后CD4+T细胞绝对计数分为A(CD4+<200 cells/μl)、B(200≤CD4+≤349 cells/μl)、C(CD4+≥350 cells/μl)3组,考察3组间T细胞亚群的差别。结果:HIV-1前病毒DNA的log拷贝数与CD4+CD45RA+T细胞绝对计数呈负相关(r=-0.231,P<0.05),与CD4+CD45RA+T细胞相对计数呈明显负相关(r=-0.270,P<0.01);与CD38+T细胞绝对计数呈正相关(r=0.250,P<0.05);与HAART持续治疗时间无相关性。B、C组的CD3+T细胞绝对计数明显高于A组(P<0.01);C组的CD8+T细胞绝对计数高于B组的(P<0.05);B、C组的CD4+CD28+T细胞绝对计数和相对计数明显高于A组(P<0.01),C组的CD4+CD28+T细胞绝对计数高于B组(P<0.05);B、C组的CD4+CD45RA+T细胞、CD4+CD45RO+T细胞绝对计数明显高于A组(P<0.01),C组的CD4+CD45RA+T细胞、CD4+CD45RO+T细胞绝对计数高于B组(P<0.05),B、C组的CD4+CD45RO+T细胞相对计数高于A组(P<0.05);B、C组的CD8+CD38+T细胞绝对计数低于A组(P<0.05),B组的CD8+CD38+T细胞相对计数低于A组(P<0.05);C组的CD38+T细胞绝对计数高于A组(P<0.05)。A、B、C组的HIV-1前病毒DNA的log拷贝数分别为3.561±0.297 9,3.605±0.277 6,3.434±0.289 1(copies/ml),3组间无显著性差异(P>0.05)。结论:经过HAART治疗后HIV-1前病毒DNA可能处于稳定状态,HIV-1前病毒DNA拷贝数只是某些T细胞亚群数量改变的原因之一。

PBMC HIV-1 DNA的动态监测在HIV-1感染者抗病毒治疗过程中的临床意义

目的探讨1型艾滋病病毒(HIV-1)感染者接受抗病毒治疗(ART)过程中,当获得核糖核酸(RNA)病毒学完全抑制后,患者外周血单个核细胞(PBMC)中HIV-1脱氧核糖核酸(DNA)的动态变化及其临床意义。方法分别在HIV-1感染者血浆HIV-1 RNA首次<20拷贝/mL时(定义为转阴)、RNA转阴1年时、RNA转阴2年时检测患者PBMC中HIV-1 DNA的含量,比较三个时间点患者PBMC中HIV-1 DNA含量的动态变化,不同ART方案以及获得RNA病毒学完全抑制所需的时间对HIV-1感染者PBMC中HIV-1 DNA的影响。结果治疗组34例HIV-1感染者接受ART过程中,在血浆HIV-1 RNA首次转阴时、RNA转阴1年时、RNA转阴2年时三个时间点患者PBMC中HIV-1 DNA含量分别为(2.88±0.50)、(2.58±0.47)、(2.57±0.43)Log10拷贝/106个细胞,差异有统计学意义;而未接受ART的对照组15例HIV-1感染者PBMC中HIV-1 DNA含量为(3.26±0.56)Log10拷贝/106个细胞,与ART治疗组比较,差异有统计学意义;含依非韦伦的一线方案和含洛匹那韦/利托那韦的二线方案对患者PBMC中HIV-1 DNA含量的影响无明显统计学差异;HIV-1感染者获得RNA病毒学完全抑制的时间越早,其PBMC中HIV-1 DNA的水平越低。结论在ART获得RNA病毒学完全抑制的HIV-1感染者仍可检出PBMC HIV-1 DNA;随着ART延长,PBMC HIV-1 DNA逐渐消减;PBMC HIV-1 DNA检测有助于判断ART疗效。

治疗性HIV-1重组DNA疫苗的构建与免疫效果评价

目的 构建编码HIV- 1多表位抗原基因 (MEG)与p2 4基因嵌合的核酸疫苗 ,并评价其免疫效果。方法 将编码HIV -1多表位抗原基因 (MEG)与p2 4基因插入到真核表达载体pVAXI中 ,构建HIV- 1治疗性重组核酸疫苗质粒。通过ELISA试剂盒检测免疫恒河猴血清中HIV -1特异性抗体 ,并通过淋巴细胞转化实验检测HIV -1特异性T淋巴细胞增殖反应。结果 构建的重组核酸疫苗质粒pVAXI -MEGp2 4免疫恒河猴后 ,能有效地刺激产生T淋巴细胞特异性增殖反应 ,并诱导产生抗HIV -1特异性抗体。结论 所构建的重组核酸疫苗质粒能诱导机体产生免疫反应。