Three amino acid residues in the envelope of human immunodeficiency virus type 1 CRF07_BC regulate viral neutralization susceptibility to the human monoclonal neutralizing antibody IgG1b12

The CD4 binding site(CD4bs) of envelope glycoprotein(Env) is an important conserved target for anti-human immunodeficiency virus type 1(HIV-1) neutralizing antibodies. Neutralizing monoclonal antibodies IgG1 b12(b12) could recognize conformational epitopes that overlap the CD4 bs of Env. Different virus strains, even derived from the same individual, showed distinct neutralization susceptibility to b12. We examined the key amino acid residues affecting b12 neutralization susceptibility using single genome amplification and pseudovirus neutralization assay. Eleven amino acid residues were identified that affect the sensitivity of Env to b12. Through site-directed mutagenesis, an amino acid substitution at position 182 in the V2 region of Env was confirmed to play a key role in regulating the b12 neutralization susceptibility. The introduction of V182 L to a resistant strain enhanced its sensitivity to b12 more than twofold. Correspondingly, the introduction of L182 V to a sensitive strain reduced its sensitivity to b12 more than tenfold. Amino acid substitution at positions 267 and 346 could both enhance the sensitivity to b12 more than twofold. However, no additive effect was observed when the three site mutageneses were introduced into the same strain, and the sensitivity was equivalent to the single V182 L mutation. CRF07_BC is a major circulating recombinant form of HIV-1 prevalent in China. Our data may provide important information for understanding the molecular mechanism regulating the neutralization susceptibility of CRF07_BC viruses to b12 and may be helpful for a vaccine design targeting the CD4 bs epitopes.

Construction and expression of an optimized, novel human immunodeficiency virus type-1 lentiviral vector containing green fluorescent protein

The human immunodeficiency virus （HIV） lentiviral vector is an ideal vector for gene therapy. In the present study, the wild-type HIV-1 genome was segregated into four plasmids, and an optimized novel HIV-1 lentiviral vector containing green fluorescent protein and vesicular stomatitis virus G pseudo-capsule was constructed. The plasmids were pHR-CMV-EGFP, pCMVΔ8.9, pRSV-Rev, pCMV-VSV-G. The four plasmid system was co-transfected into 293T cells, and green fluorescent protein expression was observed. The present study obtained lentiviral particles by high-speed centrifugation, and the lentiviral particle titer was 4 × 108 TU/mL after centrifugation. Thus, an optimized novel HIV-1 lentiviral vector was successfully constructed.

INTRACELLULAR EXPRESSION OF MULTIMERIZED ANTISENSE TAR-CORE RNAS INHIBIT THE REPLICATION OF HUMAN IMMUNODEFICIENCY VIRUS TYPE 1 IN HUMAN CD_4+T LYMPHOCYTES

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The in vitro inhibitory effect of human neutrophil peptide-1 on human immunodeficiency virus type 1

In order to clarify the mechanism of inhibition of human neutrophil peptide-1 （HNP-1） on human immunodeficiency virus type 1（HIV-1）, CD4+ cells were used as the target cells for acute infection with HIV-1, and experiments were performed separately with the interaction of different concentrations of HNP-1 with free virus particles, un-infected and infected CD4+ cells. The activity of reverse transcriptase （RT） in the supernatant of cell cultures of different lots of experiments were then assayed accordingly, and the toxicity effect on human lymphocytic cells MT4 was measured by MTT assay. The experimental results showed that pre-incubation of HNP-1 with the concentrated stock of virus could block the binding of virus to target cells with EC50 of 2.49 μg/ml, while pre-treatment of CD4+ cells with HNP-1 prior to inoculation could reduce the ability of cells to bind virus with EC50 of 20.7 μg/ml. In addition, When culturing the infected CD4+ cells in the continuous presence of various concentrations of HNP-1 added immediately after infection, HNP-1 exhibited modest inhibitory effect on viral replication with reduced RT activities in comparison with those of the control group （P<0.05 at 100 μg/ml of the highest concentration）. No cytotoxicity effect of HNP-1 was observed as demonstrated by MTT assay. These results indicate that HNP-1 exerts anti-HIV activity by at least two levels: direct inactivation of virus particles and effect on the ability of target cells to bind with viruses. The evaluation of two parameters, inhibitory effect and the cytotoxicity renders HNP-1 an available candidate for anti-HIV therapeutic agent.

Cost and safety of assisted reproductive technologies for human immunodeficiency virus-1 discordant couples

Due to significant advances in the treatment of human immunodeficiency virus type-1(HIV-1), HIV-1 infection gradually has become a treatable chronic disease. Successfully treated HIV-positive individuals can have a normal life expectancy. Hence, more and more HIV-1 discordant couples in Taiwan and the rest of the world are seeking fertility assistance. Pre-treatment of highly active antiretroviral therapy(HAART) combined with sperm washing and RT-polymerase chain reaction examination for HIV-1 viral load has become the standard procedure to assist them to conceive. However,in order to reduce the transmission risk to the lowest level for the couple and to diminish the cost of health care for the insurance institutes or government, in vitro fertilization(IVF)-intracytoplasmic sperm injection(ICSI) therapy provides the ideal solution for HIV-1 discordant couples with infected men. Intrauterine insemination(IUI) theoretically introduces more than 107 times of sperm counts or semen volume to uninfected women vs IVF-ICSI. However, since some regimens of HAART may significantly decrease the sperm motility, compared to IVF-ICSI, IUI only produces 1/5 to 1/2 pregnancy rates per cycle. Given the risk of seroconversion of HIV infection which actually happens after successful treatment, IVF-ICSI for these HIV-1 seropositive men is more cost-effective and should be the first line treatment for these cases.

Improvement in human immunodeficiency virus-1/acquired immune deficiency syndrome patients' well-being following administration of “Phyto V7”

AIM:To corroborate the capacity of Phyto V7,a complex of phytochemicals,to improve the physical well-being of human immunodeficiency virus-1(HIV-1) infected and acquired immune deficiency syndrome(AIDS) patients not undergoing antiretroviral treatment.METHODS:Two hundred and thirty nine HIV-1 seropositive male and female voluntary inmates were recruited through the Uruguay National Program of AIDS.The study participants received for 90 consecutive days every eight hours two tablets(760 mg/each) of Phyto V7,containing a mix of the following phytochemicals:flavonols(Kaempferol,Quercetin),flavones(Apigenin,Luteolin),hydroxycinnamic acids(ferrulic acid),carotenoids(Lutein,Lycopene,Beta carotene) and organosulfur compounds,all from vegetal origin.The participants did not receive any antiretroviral treatment during the study.At days 0,30,60 and 90(± 2 d) the participants were evaluated for body mass index(BMI),tolerance to Phyto V7 and Index of Quality of Life based on the Karfnosky scale.ANOVA,Tukey Post-test,χ2 test and Wilcoxon Signed Rank test were used to analyze the effect of treatment.RESULTS:One hundred and nighty nine study participants finished the study.Already after 30 d of Phyto V7 consumption,the weight,BMI and Karnofsky score statistically significantly improved(P < 0.001),and continued to improve until the end of the study.The mean weight gain per participant during the 90 d wasof 1.21 kg(approximately 2% of body weight).The overall increase in the mean Karnofsky score after 90 d was 14.08%.The lower the BMI and Karnofsky score of the participants were at the beginning of the study,the more notorious was the improvement over time.For example,the mean increment of Index of Quality of Life,among the participants with an initial Karnofsky score of 5 or below(n = 33) from day 0 to day 90,was of 35.67%(0.476 ± 0.044 vs 0.645 ± 0.09; P < 0.001).The tolerability to Phyto V7 was very good and no adverse reactions were recorded or reported.CONCLUSION:Administration of the Phyto V7 can be an important tool to improve the well-being of HIV-1 seropositive individuals and AIDS patients,not undergoing antiretroviral treatment.

HIV-1整合酶基因序列分析方法验证

目的 验证实验室自建人类免疫缺陷病毒1型(HIV-1)整合酶基因序列分析方法。该方法可用于评估HIV-1整合酶区段基因型耐药水平。方法 根据世界卫生组织自建基因序列分析方法验证的建议,从20份HIV-1阳性样本中提取RNA,扩增HIV-1整合酶区基因片段,并测序。通过与病毒质量保证(VQA)共识进行比对,评估实验室自建的HIV-1整合酶基因序列分析方案的准确性,通过扩增成功率评估其灵敏度,通过同一样本的重复检测结果评估其精密度和重现性。结果 20份样本与VQA共识的核苷酸一致率均>98%;10个高病毒载量(>10 000拷贝·mL^(-1))样本和5个低病毒载量(1 000~5 000拷贝·mL^(-1))样本的扩增成功率均为100%;4个样本的同批次5复孔和5个样本5次检测的结果均符合90%的样本配对比较核苷酸一致率>98%的要求。结论 该HIV-1整合酶基因序列分析方法的准确性、灵敏度、精密度和重现性均符合要求,适用于HIV-1整合酶基因序列分析。

The role of monocyte-lineage cells in human immunodeficiency virus persistence: mechanisms and progress

Human immunodeficiency virus type 1(HIV-1) persistence is a major barrier to the successful treatment and eradication of acquired immunodeficiency syndrome(AIDS).In addition to resting CD4+ T cells,a significant long-lived compartment of HIV-1 infection in vivo includes blood monocytes and tissue macrophages.Studying HIV-1 persistence in monocyte-lineage cells is critical because these cells are important HIV-1 target cells in vivo.Monocyte-lineage cells,including monocytes,dendritic cells(DCs) and macrophages,play a significant role in HIV-1 infection and transmission.These cells have been implicated as viral reservoirs that facilitate HIV-1 latency and persistence.A better understanding of HIV-1 interactions with monocyte-lineage cells can potentially aid in the development of new approaches for intervention.This minireview highlights the latest advances in understanding the role of monocyte-lineage cells in HIV-1 persistence and emphasizes new insights into the mechanisms underlying viral persistence.

Human T-lymphotropic virus type 1-associated myelopathy/tropical spastic paraparesis: Clinical presentation and pathophysiology

Human T-cell lymphotropic virus type 1(HTLV-1)-associated myelopathy/tropical spastic paraparesis(HAM/TSP) is a slowly progressive neurodegenerative disorder in which lesions of the central nervous system cause progressive weakness, stiffness, and a lower limb spastic paraparesis. In some cases, polymyositis, inclusion bodymyositis, or amyotrophic lateral sclerosis-like syndromes are associated with HTLV-1. TSP was first described in Jamaica in 1888 and known as Jamaican peripheral neuritis before TSP was related to HTLV-1 virus, the first retrovirus being identified, and the disease is since named HAM/TSP. There is no established treatment program for HAM/TSP. Prevention is difficult in lowincome patients(i.e., HTLV-1 infected breast feeding mothers in rural areas, sex workers). Thus, there is a need for new therapeutic avenues. Therapeutic approaches must be based on a better understanding, not only of clinical and clinicopathological data, but also of the pathophysiology of the affection. Consequently, a better understanding of existing or newly developed animal models of HAM/TSP is a prerequisite step in the development of new treatments.

Post-transcriptional gene silencing, transcriptional gene silencing and human immunodeficiency virus

While human immunodeficiency virus 1(HIV-1) infectionis controlled through continuous, life-long use of a combination of drugs targeting different steps of the virus cycle, HIV-1 is never completely eradicated from the body. Despite decades of research there is still no effective vaccine to prevent HIV-1 infection. Therefore, the possibility of an RNA interference(RNAi)-based cure has become an increasingly explored approach. Endogenous gene expression is controlled at both, transcriptional and post-transcriptional levels by noncoding RNAs, which act through diverse molecular mechanisms including RNAi. RNAi has the potential to control the turning on/off of specific genes through transcriptional gene silencing(TGS), as well as finetuning their expression through post-transcriptional gene silencing(PTGS). In this review we will describe in detail the canonical RNAi pathways for PTGS and TGS, the relationship of TGS with other silencing mechanisms and will discuss a variety of approaches developed to suppress HIV-1 via manipulation of RNAi. We will briefly compare RNAi strategies against other approaches developed to target the virus, highlighting their potential to overcome the major obstacle to finding a cure, which is the specific targeting of the HIV-1 reservoir within latently infected cells.

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.

A Human T Lymphotropic Virus Type 1 Carrier Coinfected with <i>Mycobacterium intracellulare</i>and <i>Pneumocystis jirovecii</i>with a Characteristic Compositional Change of Bone Marrow Cells

Human T lymphotropic virus type 1 (HTLV-1) is endemic in the southern part of Japan. Infection of the virus can cause adult T cell leukemia/lymphoma (ATL), while most infected individuals remain in a carrier state for a long period of time. Although rare cases of carriers, like ATL patients, who developed opportunistic infections, have been reported, hematological changes of carriers who are prone to opportunistic infections have not been well defined. Here, we present a case of an HTLV-1 carrier who developed Mycobacterium intracellulare infection and Pneumocystis jirovecii pneumonia (PcP) simultaneously. Flow cytometric analysis of bone marrow cells revealed an aberrant compositional change similar to that in ATL patients. This suggests the presence of a pre-ATL state prior to the development of ATL, which is notable in terms of underlying cellular immunodeficiency.

水芹总酚酸体外抗HIV-1的作用

目的探讨水芹总酚酸体外抑制人类免疫缺陷病毒1型的作用。方法用不同稀释度的水芹总酚酸与TZM-bl细胞共同培养,使用MTT法检测活细胞的数量,观察水芹总酚酸对TZM-bl细胞的毒性作用;用人类免疫缺陷病毒1型实验室适应株SF33、BAL分别感染TZM-bl细胞,基于TZM-bl细胞的荧光素酶检测体系,采用荧光素酶活性检测方法检测水芹总酚酸抗人类免疫缺陷病毒1型的活性。结果水芹总酚酸对TZM-bl细胞表现出较低的细胞毒性,半数细胞毒浓度>1600μg·ml^(-1)。水芹总酚酸对TZM-bl细胞HIV-1 SF33、HIV-1 BAL病毒的半抑制浓度平均值分别为38.93和24.25μg·ml^(-1),治疗指数分别为>41和>66。结论水芹总酚酸在体外具有抑制人类免疫缺陷病毒1型复制活性的作用。

芒果叶提取物体外抗HIV-1活性研究

目的探讨芒果叶提取物的体外抗人类免疫缺陷病毒1(HIV-1)活性,为研究与开发传统中医药资源治疗获得性免疫缺陷综合征(AIDS)提供参考。方法通过三磷酸腺苷(ATP)法评估干预药物对TZM-bl细胞和MT-2细胞活性的影响。构建TZM-bl-HIV-1_(ⅢB)、MT-2-HIV-1_(ⅢB)两种细胞-病毒感染模型,通过荧光素酶活性检测试剂检测病毒活性,评估干预药物的抗HIV-1活性。观察MT-2-HIV-1_(ⅢB)细胞系统中芒果叶提取物对细胞病变效应(CPE)的抑制情况。计算芒果叶提取物的半数毒性浓度(CC_(50))、半数抑制浓度(IC_(50))和选择指数(SI)。结果在TZM-bl-HIV-1_(ⅢB)和MT-2-HIV-1_(ⅢB)两种细胞-病毒感染模型中,芒果叶提取物均显示出抗HIV-1活性,且呈现剂量依赖性。在TZM-bl-HIV-1_(ⅢB)模型中,芒果叶提取物的CC_(50)为(320.00±29.44)μg/ml,IC_(50)为(8.86±0.26)μg/ml,SI为36.14。在MT-2-HIV-1_(ⅢB)模型中,芒果叶提取物CC_(50)为(174.13±22.36)μg/ml,IC_(50)为(15.23±9.99)μg/ml,SI为11.44。结论芒果叶提取物的体外细胞毒性小,抗HIV-1活性显著,具有潜在的开发利用价值。

湖南省HIV-1感染者原发性耐药现况调查

目的了解湖南省1型人类免疫缺陷病毒(HIV-1)感染者其基因亚型分布和原发性耐药(PDR)情况,为艾滋病防控及抗病毒治疗(ART)提供参考依据。方法收集湖南省2021年1月—2022年8月某院HIV门诊新确诊并且未接受ART的HIV-1感染者的人口学及流行病学相关数据,采集患者血清,提取核糖核酸,利用In-house的方法采取2轮聚合酶链式反应进行基因扩增,Sanger法对产物进行测序,分析患者临床资料及HIV-1亚型及耐药情况。结果共纳入患者667例,基因型耐药检测失败20例,647例检测成功的新确诊HIV-1感染者纳入研究。53例患者感染的HIV-1株发生PDR,发生率为8.19%,主要集中于男性(88.68%)、未婚(71.70%)、男男性行为(MSM,60.38%)、21~40岁的群体(58.49%),且多为湖南省本地籍居民(98.11%)。共检测出15种HIV-1毒株亚型,主要亚型为CRF_01AE(35.70%)、CRF07_BC(25.19%)、B/C(18.86%)以及CRF55_01B(7.88%)。不同HIV-1亚型患者的PDR发生率比较,差异有统计学意义(χ^(2)=18.62,P=0.017)。蛋白酶抑制剂(PIs)耐药率为0.15%,核苷酸类逆转录酶抑制剂(NRTIs)耐药率为2.78%,非核苷酸类逆转录酶抑制剂(NNRTIs)耐药率为6.65%,整合酶抑制剂(INSTIs)耐药率为0.31%。结论湖南省HIV-1毒株亚型分布复杂,PDR发生率已超过世界卫生组织制定的低水平耐药预警线(<5%),应加大感染预防与控制力度,阻断耐药毒株传播。

HIV-1感染患者外周血单核细胞miR-20a、miR-122表达与HIV-1 DNA、HIV-1 RNA及CD4+T淋巴细胞计数的关系

目的检测人类免疫缺陷病毒-1(HIV-1)感染者外周血单个核细胞(PBMCs)微小RNA(miR)-20a、miR-122表达水平,探讨其与HIV-1 DNA、HIV-1 RNA及CD4+T淋巴细胞计数关系。方法选取2021年5月~2023年1月南通市第三人民医院收治的HIV-1感染患者110例作为HIV-1组,依据HIV-1 DNA分为HIV-1 DNA高表达组(DHG组,n=65例)、HIV-1 DNA低表达组(DLG组,n=45例);依据HIV-1 RNA分为HIV-1 RNA高表达组(RHG组,n=49例)、HIV-1 RNA低表达组(RLG组,n=61例);根据CD4+T淋巴细胞计数分为<200 cellsμl组(n=36例)、200~350 cellsμl组(n=48例)、>350 cellsμl组(n=26例)。另选取同时间段健康体检者110例作为健康对照组。荧光定量PCR法检测PBMCs miR-20a、miR-122、HIV-1 DNA以及血浆HIV-1 RNA,流式细胞仪获取CD4+T淋巴细胞计数。比较各组患者PBMCs中miR-20a、miR-122水平差异。Pearson法分析两指标间相关性。结果HIV-1组PBMCs中miR-20a、miR-122水平高于健康对照组[(1.72±0.45)vs.(1.09±0.12)、(1.51±0.38)vs.(1.04±0.07)],差异有统计学意义(t=14.188、12.757,P<0.05)。与DLG组相比,DHG组患者PBMCs中miR-20a、miR-122水平均明显升高[(1.91±0.48)vs.(1.45±0.41)、(1.64±0.39)vs.(1.32±0.37)],差异有统计学意义(t=5.239、4.320,P<0.05)。RHG组PBMCs中miR-20a、miR-122水平高于RLG组[(1.85±0.46)vs.(1.62±0.44)、(1.70±0.40)vs.(1.36±0.36)],差异有统计学意义(t=2.670、4.685,P<0.05)。<200 cellsμl组、200~350 cellsμl组、>350 cellsμl组miR-20a、miR-122水平逐次降低[(2.04±0.55)、(1.67±0.46)、(1.37±0.29),(1.73±0.40)、(1.51±0.39)、(1.21±0.33)],差异有统计学意义(F=16.525,14.117,P<0.05)。相关性结果显示,HIV-1组PBMCs中miR-20a与miR-122呈正相关(r=0.651,P<0.05),miR-20a、miR-122均与HIV-1 DNA(log 2 DNA)有明显正相关(r=0.569、0.471,P<0.05),与HIV-1 RNA(log 2 RNA)有明显正相关(r=0.491、0.444,P<0.05),但与CD4+T淋巴细胞计数呈负相关性(r=-0.555、-0.536,P<0.05)。结论HIV-1感染者PBMCs中miR-20a、miR-122表达水平升高,与CD4+T淋巴细胞计数及HIV-1病毒的DNA和RNA定量检测结果相关,可能与病毒储存库建立有关,检测二者水平可反映患者感染状况。

环索奈德通过靶向HIV-1衣壳蛋白六聚体调节其体外装配

多肽CAI在HIV-1衣壳蛋白(CA)C末端的结合口袋可用来筛选CA蛋白装配调节剂。采用均相时间分辨荧光技术(HTRF)筛选399个化合物,发现1个小分子化合物环索奈德(ciclesonide)能够竞争性抑制十二肽CAI与CA蛋白C末端的结合,其半数抑制浓度IC_(50)值为6.06μmol/L。生物膜干涉技术(BLI)测量环索奈德与CA蛋白(单体和六聚体)的结合,环索奈德与CA六聚体的亲和力为159 nmol/L,远远大于其与CA单体的亲和力(K_(D)=1.68 mmol/L)。衣壳蛋白体外装配实验表明,环索奈德能促进CA蛋白的装配,且具有浓度依赖性。分子模拟分析环索奈德与CA蛋白的结合模式,显示环索奈德与CA六聚体的相互作用发生在六聚体相邻亚基N末端-C末端的界面上,并与H67和L211两个残基形成氢键。研究表明,环索奈德是一种潜在的HIV-1衣壳装配调节剂。

Primary Effusion Lymphoma in a HIV-1/2-Infected Patient

Background: Primary effusion lymphoma (PEL) is a lymphoid proliferation related to Kaposi sarcoma herpesvirus 8/human herpesvirus 8 (KSHV/HHV8) that affects mainly human immunodeficiency virus (HIV) infected individuals but can also occur in other immunodeficiency settings. It is characterized by lymphomatous effusions in different serous body cavities without the presence of a detectable tumor mass. The diagnosis is challenging and the clinical outcomes are poor. Aim: The aim of this paper is to report a rare case of PEL in a man who have sex with women (MSW) with HIV-1/2 infection, history of visceral Kaposi sarcoma (KS) and the development of a seronegative arthritis previous to the lymphoproliferative disease diagnosis. PEL presented with ascites, was treated with high-dose chemotherapy and autologous stem cell transplantation, with a good clinical outcome. Case Presentation: We describe a case of a 48-year-old HIV-1/2-infected patient from a high HHV8 seroprevalent country, hospitalized following a three-month history of increased abdominal volume and general constitutional symptoms. Laboratory data revealed normocytic normochromic anemia and a high level of lactate dehydrogenase. A diagnostic paracentesis was performed with cytology compatible with high-grade B-cell lymphoma. Peritoneal fluid cytology showed large lymphoid cells expressing leucocyte-common antigen CD45 without expression of the CD20 antigen (B-lymphocytes) and positivity for HHV8 by immunocytochemical staining, compatible with the diagnosis of PEL.

Differential selection in HIV-1 gp120 between subtype B and East Asian variant B'

HIV-1 evolves strongly and undergoes geographic differentiation as it spreads in diverse host populations around the world.For instance,distinct genomic backgrounds can be observed between the pandemic subtype B,prevalent in Europe and North-America,and its offspring clade B' in East Asia.Here we ask whether this differentiation affects the selection pressure experienced by the virus.To answer this question we evaluate selection pressure on the HIV-1 envelope protein gp120at the level of individual codons using a simple and fast estimation method based on the ratio k_alk_s of amino acid changes to synonymous changes.To validate the approach we compare results to those from a state-of-the-art mixed-effect method.The agreement is acceptable,but the analysis also demonstrates some limitations of the simpler approach.Further,we find similar distributions of codons under stabilizing and directional selection pressure in gp120 for subtypes B and B' with more directional selection pressure in variable loops and more stabilizing selection in the constant regions.Focusing on codons with increased k_alk_s values in B',we show that these codons are scattered over the whole of gp120,with remarkable clusters of higher density in regions flanking the variable loops.We identify a significant statistical association of glycosylation sites and codons with increased k_alk_s values.

福建省HIV-1流行毒株基因分型与流行特征分析

目的了解HIV-1流行株在福建省感染人群中的基因亚型分布及流行特征。方法随机抽取福建省2003-2005年发现的70例HIV感染者血样,提取前病毒DNA进行体外扩增,获得核心蛋白(gag)、包膜蛋白(env)及pol区基因的核酸片段,并对各基因区核苷酸序列进行测定和序列分析。结果选取46份流行病学资料以及不同基因区域序列资料完整的样本进入亚型分析,结果显示目标人群中存在B、C2种亚型以及CRF07-BC、CRF08-BC、CRF01-AE3种流行重组型,以及国内未见报道的B/F重组毒株、A1/D重组毒株等,其中以CRF01-AE重组毒株为主,占69.56%。基因亚型的流行特征分析显示,本省感染的HIV患者中以CRF01-AE重组型占多数,可能的新型重组型全部分布于境外感染者中;在性接触传播的感染者(71.74%)中呈现多种亚型分布的特征;随着时间变化福建省HIV感染者的亚型分布发生变化。结论福建省HIV-1亚型分布众多,各亚型在不同感染地分布不平衡,性乱人群中的亚型分布较为复杂,从总的亚型流行特征来看,HIV-1在我省有流行加快的趋势。