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GBV-C/HGV and HIV-1 coinfection

Abstract

An interesting interaction pattern has been found between HIV-1 and GBV-C/HGV, resulting in protection against progression to AIDS. The mechanisms involved in this interaction remain to be clarified. We examined the current knowledge concerning this coinfection and developed hypotheses to explain its effects. A better understanding of this interaction could result in new concepts, which may lead to new strategies to control HIV-1 replication and progression to AIDS.

HIV; HGV; GBV-C; pathogenesis; review


MINI-REVIEWS

GBV-C/HGV and HIV-1 coinfection

Maria Teresa MaidanaI; Ester Cerdeira SabinoII; Esper Georges KallasI

IFederal University of São Paulo

IIPró-Sangue Foundation; São Paulo, SP, Brazil

Correspondence Correspondence to Dr. Esper Georges Kallas, M.D., Ph.D Laboratório de Imunologia, Disciplina de Doenças Infecciosas e Parasitárias, Escola Paulista de Medicina / UNIFESP Rua Pedro de Toledo 781, 15º andar Zip code: 04039-032 - São Paulo - SP, Brazil E-mail: kallas.dmed@epm.br

ABSTRACT

An interesting interaction pattern has been found between HIV-1 and GBV-C/HGV, resulting in protection against progression to AIDS. The mechanisms involved in this interaction remain to be clarified. We examined the current knowledge concerning this coinfection and developed hypotheses to explain its effects. A better understanding of this interaction could result in new concepts, which may lead to new strategies to control HIV-1 replication and progression to AIDS.

Key Words: HIV, HGV, GBV-C, pathogenesis, review

Patients infected with the human immunodeficiency virus (HIV) are often co-infected with other pathogens, especially hepatitis viruses [1]. Coinfection with hepatitis B virus (HBV) or hepatitis C virus (HCV) appears to increase the mortality rate among HIV-infected patients [2], in the same way as the course of HCV infection is accelerated in patients who are coinfected with HIV, when compared with immunocompetent individuals [3,4]. A new virus related to hepatitis C virus was identified in 1995; it was initially thought to be another hepatitis agent [5,6]. It has been described as either GB virus C (GBV-C) [5] or hepatitis G virus (HGV) [6]. GBV-C and HGV are closely related, with more than 95 percent sequence homology [7]. The name GBV-C has been more widely used, since it appears that this virus is not a causative agent of hepatitis [7,8].

GB virus C (GBV-C), an RNA virus in the Flaviviridae family, has a genome very similar to that of hepatitis C virus (HCV), coding for structural and nonstructural proteins. There is a nontranslated region (NTR) at 5' that can serve as an internal ribosomal entry site to direct translation of the uncapped message (genome) RNA [9]. GVB-C appears to encode two structural glycoproteins, which constitute the virus envelope proteins E1 and E2. However, the precise composition of the nucleocapsid has yet to be defined. To date, five genotypes of HGV have been described, with 12 percent divergence between them [10,11]. Genotype 1 is predominant in West Africa, genotype 2 in Europe and the USA, genotype 3 in Asia, genotype 4 in Southeast Asia and genotype 5 in South Africa [12]. In Brazil, two reports have described the genotype distribution. Oliveira et al. evaluated 17 GVB-C-infected blood donors using RFLP, of which 10 (59%) were infected by genotype 2b, four infected by genotype 2a (24%), and three by genotype 1 (18%) [13]. Nishiya et al. screened over 1,000 healthy subjects, and analyzed 24 GVB-C-infected patients, using RT-PCR followed by genome sequencing; they found 12 subjects infected by genotype 2a (50%), 10 by genotype 2b (42%), and two by genotype 1 (8.3%) [14].

Although many people are infected with this virus throughout the world, no clear association with a known disease state has been demonstrated. GBV-C is transmitted predominantly through parenteral routes, with a high seroprevalence among intravenous illicit drug users, although sexual transmission has also been reported [15].

Based on the very low density of the virus particles, it appears that GBV-C associates with lipids in human serum, and like HCV, it may use the low density lipoprotein receptor for virus binding and entry into target cells [16]. Virus derived from an infectious molecular clone can replicate in CD4+ cells in peripheral blood mononuclear cell (PBMC) cultures [17].

GBV-C clearance is common in immunocompetent subjects, occurring in approximately 60 to 75% of GBV-C-infected persons, along with the development of antibodies against the envelope glycoprotein E2 [18]. GBV-C infection has not been associated with any known disease and does not appear to represent a substantial threat to public health. For this reason, the Food and Drug Administration (FDA) has not recommended screening blood donors for GBV-C RNA, although this persistent infection is common, present in approximately 1.8% of American donors and more than 35% of the HIV-infected subjects [19]. In Brazil, the prevalence of HGV in blood donors is higher, being around 9% [20]. In a study conducted in a representative sample of the city of São Paulo, it was found that the prevalence varies according to the age group, peaking in individuals between 30 and 40 years old. The prevalence in children between 5 and 9 years old was found to be high (2.9%), suggesting that other transmission routes, besides parenteral and sexual, are important in this age group [21].

Whereas the presence of antibodies against the envelope protein E2 (anti-E2) indicates viral clearance, the presence of GBV-C RNA in serum or plasma indicates ongoing GBV-C infection [22]. GBV-C RNA can be detected by nucleic acid amplification systems [23-25], and quantification has been accomplished using branched chain DNA assays [26] and real-time (Taq Man) polymerase chain reaction (PCR).

GBV-C viremia is associated with a lower mortality rate among HIV-1 infected patients, slower progression to AIDS, and longer survival once AIDS has developed [26-29]. In another study, these effects were found to be independent of age, HIV-1 load, HCV load, CD4+ and CD8+ T cell counts, and CC chemokine receptor 5 (CCR5) genotype [30]. It was also observed that serum levels of interleukin-2 (IL-2), IL-12, IL-4, and IL-10 remained relatively stable over time in the GBV-C RNA-positive group, while the GBV-C RNA negative group had a decrease in IL-2 and IL-12 of approximately 85% and 83%, respectively, and IL-4 and IL-10 increased by 654 and 395%, respectively, preserving a TH1 cytokine response [29].

GBV-C virus did not prevent the entry of HIV in the cell or the depletion of T CD4+ cells, but it did have an inhibitory effect in replication and HIV growth in cell culture [31]. This effect did not appear to be a result of cellular toxicity, considering that GBV-C replication in peripheral-blood mononuclear cells appeared to be noncytopathic and did not inhibit the synthesis of cellular proteins [31].

Over the past several years, there has been substantial controversy over the interactions between GBV-C and HIV in vivo. A number of studies have demonstrated a surprising survival benefit among patients who are coinfected, when compared with those who are only infected with HIV-1. Other studies, however, have not shown such effects. The article by Williams et al. [32] may settle a few aspects of this controversy, since it clearly demonstrates that five to six years after HIV-1 seroconversion patients were more likely to be dead if they were infected only with HIV-1 than if they were coinfected with both HIV-1 and GBV-C. This significant survival advantage was not observed during the first 12 to 18 months after HIV-1 seroconversion. Likewise, the time dependence could explain the contradictory results of some studies regarding the observed protective effects of GBV-C [32].

As further evidence of the protective effect of dual infections, Williams et al. also found that the course of HIV-1 disease was adversely affected by the clearance of GBV-C viremia [32]. The mechanism of this protective effect remains to be determined and there are a number of possibilities to explain it.

In addition, some studies suggest that HIV-1 replication is directly reduced by GBV-C. The fact that both HIV-1 and GBV-C can infect and replicate within peripheral-blood mononuclear cells suggests that these two viruses interact either directly or indirectly throughout the cell cycle. Various stages of the HIV life cycle may be affected by GBV-C, including retroviral binding and fusion to target cells through the high-affinity receptor and several chemokine coreceptors, internalization and reverse transcription, integration into the host-cell genome to create the HIV provirus, viral transcription, translation and viral morphogenesis; another possibility is a series of interactions that involve CCR5.

The level of CCR5 expression is an important factor for HIV transmission and disease progression [33]. It was observed that the envelope glycoproteins of GBV-C, specifically E2, bind to CD81 on T lymphocytes. This interaction induces a dose-dependent secretion of RANTES, a natural ligand of CCR5, which induces internalization of CCR5 and down-regulation of CCR5 surface expression, with concomitant intracellular accumulation of CCR5 proteins on CD4+ and CD8+ T lymphocytes of HGV-infected subjects, at a rate of 53 and 36%, respectively. Hence, the internalization of chemokine receptors is an effective mechanism to block cellular entry of HIV into the cells [34,35]. However, it remains unclear why HGV E2 specifically induces RANTES, but not MIP-1aor MIP-1b, which are other ligands of CCR5 [36]. On the other hand, it would be of interest to know whether GBV-C clearance is associated with HIV-mediated destruction of host cells necessary for the production of GBV-C, preceding the loss of CD4+ T cells.

There is a long history of interactions between different viruses; in most cases one virus increases the pathogenicity of the other. The interaction between HIV-1 and GBV-C is unusual and curious, and it is beneficial to patients who are dually infected. It is, therefore, of great interest to understand the mechanisms involved in this interaction, because it could result in progress in our understanding of viral pathogenesis and in a contribution towards the development of novel HIV-1 treatment strategies.

Received on 17 Dezember 2004; revised 30 March 2005

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  • Correspondence to

    Dr. Esper Georges Kallas, M.D., Ph.D
    Laboratório de Imunologia, Disciplina de Doenças Infecciosas e Parasitárias, Escola Paulista de Medicina / UNIFESP
    Rua Pedro de Toledo 781, 15º andar
    Zip code: 04039-032 - São Paulo - SP, Brazil
    E-mail:
  • Publication Dates

    • Publication in this collection
      18 Aug 2005
    • Date of issue
      Apr 2005

    History

    • Reviewed
      30 Mar 2005
    • Received
      17 Dec 2004
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