![[Feedback]](/icons/banner/feedbackACT.gif){kind=icon}
![[For Subscribers]](/icons/banner/subscriberACT.gif){kind=icon}
![[Archive]](/icons/banner/archiveACT.gif){kind=icon}
![[Search]](/icons/banner/searchACT.gif){kind=icon}
![[Contents]](/icons/banner/tocACT.gif){kind=icon}
Previous Article | Next Article 
Clinical and Diagnostic Laboratory Immunology, May 1999, p. 295-305, Vol. 6, No. 3
Current Concepts in Human Immunodeficiency
Virus Infection and AIDS
Division of Allergy, Immunology, and
Rheumatology, Department of Medicine, The State University of New
York at Buffalo, Buffalo General Hospital, Buffalo, New York 14203
The global epidemic of AIDS has
become one of the most pressing public health emergencies of this
century. Initial reports of AIDS date back to 1981. However, current
data suggest that AIDS has existed for at least several decades. While
both forms of the human immunodeficiency virus (HIV), type 1 and type
2, are retroviruses capable of causing fatal AIDS, infection with the
latter generally results in a longer incubation period and a more
indolent course of disease. Maternal-fetal transmission of HIV-2 is
limited, and infection with HIV-2 seems to provide natural protection,
estimated at approximately 70%, against infection with HIV-1 in
certain high-risk groups (50). HIV-2, initially endemic to
west Africa, also is spreading worldwide.
Retroviruses encode their genetic information as RNA which, upon
infection of a host cell, is reverse transcribed into double-stranded DNA. The latter is integrated into the DNA of the host cell
chromosomes. Other examples of human retroviruses include the human
T-cell lymphotrophic viruses types I and II (HTLV-I and -II). HTLV-I is
the etiologic agent for adult T-cell leukemia and tropical spastic
paraparesis, also known as HTLV-I-associated myelopathy. Hairy cell
leukemia, a B-cell malignancy, has been linked to HTLV-II (14). HIV-1 infections produce a variety of manifestations
such as immunodeficiency with accompanying opportunistic infections, malignancies, severe cachexia, and encephalopathy including dementia (49).
Progress has been made in the treatment of HIV infections. Nucleoside
analogues that inhibited viral reverse transcriptase (RT) were the
first class of antiretroviral drugs but the emergence of resistant
strains limited their effectiveness. The recent introduction of
protease inhibitors to our current armamentarium, combined with
multidrug therapy, has yielded encouraging results (10, 13,
20). Nevertheless longitudinal outcome data, including assessment
of the emergence of drug-resistant mutants, are needed to determine the
long-term potential of current therapy.
The latest statistics provided by the Joint United Nations
Programme on HIV/AIDS (UNAIDS) record 33.4 million people living with
HIV/AIDS worldwide (1a). This can be stratified into 32.2 million adults, of whom 13.8 million are women, and 1.2 million children under the age of 15. Since the beginning of the epidemic, there has been 13.9 million deaths worldwide due to AIDS, including 3.2 million children. Within the 50 United States a cumulative total of
687,397 cases of AIDS were reported to the Centers for Disease Control
and Prevention (CDC) through the end of 1998 (12).
The first reports of AIDS in the United States occurred in June 1981. Initially, AIDS prevalence seemed to be restricted to homosexual men
and patients with hemophilia. However, HIV infections are primarily a
sexually transmitted disease (STD) that has no preference for any
sexual orientation. HIV infections may have existed for at least
several decades in central Africa, where the male to female prevalence
ratios are about equal. HIV-2 demonstrates a closer genetic
relationship and geographic distribution to the simian immunodeficiency
virus (SIV), long endemic to central Africa, than to HIV-1
(38). Sequencing studies of early HIV-2 isolates showed a
75% nucleic acid homology with SIV but only a 40 to 50% homology with
HIV-1. Thus, it was hypothesized that HIV-2 may be the prototype virus
that was originally transmitted from monkeys to man.
Transmission of HIV can occur through contact with infected body
fluids. It is currently assumed that the relatively cellular body
fluids such as blood, semen, vaginal secretions, and breast milk are
more effective in transmitting the virus than fluids deficient in cells
such as saliva, urine, and tears. Transmission may occur across mucous
membranes or broken skin during sexual intercourse (both heterosexual
and homosexual), but it also may occur via intravenous exposure such as
through sharing infected needles with intravenous drug use,
occupational exposure in the health care environment, or treatment with
infected blood products. Now that donated blood is routinely screened
for HIV in developed and many developing countries, the potential for
acquisition of HIV via this route has been reduced significantly. In
the United States recent estimates of the risk of transmission of HIV
by blood transfusion ranged from 1 in 450,000 to 1 in 660,000. The significance of exposure risk to HIV-1 is summarized in Table 1. Vertical transmission from an infected
mother to her child is a special problem. Infection can occur in utero
or intrapartum. Postpartum infection can result from the ingestion of
breast milk by a nursing infant from an infected mother
(53). It has been estimated by the World Health Organization
that up to one-third of all cases of transmission of HIV-1 from an
infected mother to her child may occur via breast milk. However, for
certain populations where the infant mortality rate is high, the risk
of death associated with the lack of breast feeding may be greater than
the risk of HIV infection acquired through breast milk (7).
1071-412X/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.
MINIREVIEW
INTRODUCTION
Top
Introduction
References
EPIDEMIOLOGY
TABLE 1.
HIV infection cases by age group, exposure category,
and sexa
| |
BIOLOGY OF HIV INFECTION |
|---|
HIV is a human retrovirus consisting of a noncomplementary pair of single coding or positive (+) strands of RNA enclosed within an inner, nucleocapsid, protein core surrounded by a lipid bilayer envelope. Various host cell proteins are incorporated into the lipid bilayer of the viral envelope. An envelope glycoprotein with a molecular size of 41 kDa (gp41) is anchored within the lipid bilayer to which gp120 is noncovalently attached (28). The crystal structure of gp120 in complex with the CD4+ receptor and a neutralizing human antibody was recently determined to a resolution of 2.5 Å (33). Figure 1 shows a diagram of the structure of HIV. The genetic map of HIV is depicted in Figure 2.
|
|
The binding of HIV to target cells was previously thought to only
involve interaction of gp120 of the virus envelope with the CD4
molecule on the cell membranes of T-helper lymphocytes, monocytes and
macrophages, and microglia in the brain (49). However,
recently it was shown that efficient viral entry requires a coreceptor
that is also the natural receptor for the 
chemokines, a family of
chemotactic cytokines (35). This will be discussed further
below. After binding, the viral envelope fuses with the membrane of the
target cell and the contents of the virus enter the cytoplasm.
Molecules of the virus-derived enzyme, RNA-dependent DNA polymerase or
RT, are released into the target cell together with the viral RNA. RT
then directs the synthesis of a complementary strand of DNA on the RNA
template from the virus. Thereafter the RT directs the synthesis of a
second strand of DNA complementary to the initial DNA strand. RT is
highly error prone through substitution of incorrect bases, accounting
for the high mutation rate of HIV. Viral nucleic acids including RNA
and DNA form a high-molecular-weight preintegration complex with HIV
proteins (e.g., RT, integrase, and matrix protein) which is transported
to the nucleus. The double-stranded DNA copy of the viral RNA is then
randomly integrated into the host's DNA. The proviral form of HIV
integrated into the host chromosome is generally quiescent and
replicates coordinately with the host cell DNA. When the HIV-infected
cell undergoes activation or stimulation, the provirus is
transactivated, resulting in the production and release of infectious
virions. The life cycle of HIV is shown in Fig.
3.
|
HIV can be broadly divided into two phenotypes: one induces syncytium formation among infected cells and the other does not (24). The syncytium-inducing (SI) strain readily infects T lymphocytes, replicates at a high rate, and is associated with a relatively more rapid course of the disease. The non-syncytium-inducing (NSI) phenotype shows tropism for macrophages, replicates slowly, and is not associated with rapid progression. The V1 and V2 loops of gp 120 regulate virus entry into the host, whereas the V3 loop is the major determinant of tropism for the SI and NSI phenotypes (31, 47, 52). Syncytium formation is enhanced in the CD45RO+ memory subset of CD4+ lymphocytes (29). Syncytia have a shorter half-life and tend to die more quickly than individual infected cells in vitro; however, this has not been demonstrated in vivo. SI strains are more frequently isolated from patients with full-blown AIDS, whereas NSI strains tend to predominant in recently infected patients. These observations suggest that the NSI phenotype is more likely to produce primary infections. This may be due to the fact that macrophages are highly susceptible to the NSI phenotype and can serve as a reservoir for HIV. In some patients, however, the asymptomatic phase may be shortened concomitant with a shift in the viral phenotype from NSI to SI. This shift in phenotype may be distinguished on the basis of CD4 counts and quantitative measurement of HIV RNA. The envelope protein of the SI strain exhibits a high affinity for the CD4+ receptor, subsequently initiating syncytium formation and target cell destruction.
Pathogenesis. Although the course of HIV-1 infection can vary widely from patient to patient, a generalized clinical course is presented in Fig. 4. Fifty to 70% of patients develop an acute mononucleosis or flu-like syndrome within 3 to 6 weeks of primary infection, characterized by high levels of viremia and a significant drop in the absolute number of CD4+ cells in the peripheral blood. The acute viremia is followed by activation of CD8+ cells, which may be a response to control virus replication by cytotoxicity against infected target cells or through production of a soluble mediator that can suppress viral replication. During this stage, HIV is widely disseminated to the lymph nodes and induces a rapid turnover of infected lymphocytes (32, 49). It has been estimated from a mathematical model that the rate of virus production during active infection with HIV-1 is 10.3 × 109 virions per day, and productively infected cells have a life-span of 2.2 days (22, 44). The extraordinary high production of virions and the disproportionate daily loss of CD4+ cells led to what has become known as the "sink model" for CD4+ cell loss (2).
|
Apoptosis. Earlier studies implicated a variety of mechanisms in the progressive depletion of the absolute number of CD4+ cells in the peripheral blood of patients with HIV infection. These included syncytium formation between infected and uninfected CD4+ cells, selective infection or destruction of memory T cells, killing of uninfected cells by an autoimmune mechanism, Fc receptor-mediated antibody-dependent cellular cytotoxicity, and cell-mediated destruction of HIV-infected cells by cytotoxic T lymphocytes and/or NK cells. More recently another mechanism, programmed cell death or apoptosis, has been proposed to account for some of the CD4+ cell depletion observed in the peripheral blood of AIDS patients (27). Apoptosis is a physiological, cellular suicide mechanism in which cell death occurs naturally during the maturation of specific tissues or organs. Apoptosis is characterized by several morphologic and biochemical features including cell shrinkage, condensation of chromatin, and cleavage of DNA into oligonucleosome-sized (180- to 200-bp) fragments. These oligonucleosome fragments are the basis of the so-called DNA ladder formation on agarose gel electrophoresis that is a characteristic of apoptosis. Apoptosis is not restricted to only CD4+ cells in HIV infection: CD8+ T lymphocytes and B lymphocytes also undergo apoptosis (41). In HIV infection, apoptosis can be activated directly or indirectly. In indirect killing, CD4 molecules on uninfected cells can be cross-linked with gp120 of the virus envelope. This can prime the cell to undergo DNA fragmentation and subsequent programmed cell death when it encounters major histocompatibility complex (MHC) class II molecules on homologous cells or superantigens derived from various microorganisms. Regarding direct induction of apoptosis, HIV-infected cells can induce this process in uninfected cells. The activation of various genes, including fas/ApoI (CD95), Bcl-2, several protooncogenes, and tumor suppressor genes, and cytokines and transcription factors are involved in apoptosis. In HIV infection, apoptosis regulated by the expression of fas-Bcl-2 has been associated with the depletion of the CD45RO+ T cell subset (8).
T-helper lymphocyte subpopulations. Several functional subpopulations of CD4+ T-helper (Th) lymphocytes have been described including Th-1, Th-2, CD45RA+ (naive), and CD45RO+ (memory) cells. Activated Th-1 cells produce cytokines, such as gamma interferon, IL-2, and IL-12, that facilitate cell-mediated immunity. However, cytokines produced by Th-2 cells, such as IL-4, IL-5, IL-6, and IL-10, enhance humoral immune responses. Recent evidence suggests that a shift in CD4+ subpopulations from Th-1 to Th-2 predominance is associated with disease progression and clinical deterioration of HIV-infected patients (15). This hypothesis is supported by an animal model wherein mice lacking a Th-2 response resist the development of a murine form of AIDS. While this theory of Th-1 to Th-2 cell switching is not accepted by all AIDS researchers, clinical trials are under way using exogenously administered cytokines, such as IL-2, to expand the pool of CD4+ T cells and their repertoire of T-cell receptors. Although CD45RA+ and CD45RO+ markers are downregulated in HIV-1 infection, (9) an increase in the CD45RO+ subset of both CD4+ and CD8+ T cells has been associated with progression of disease (5). HIV has been shown to preferentially infect the RO+ (memory) subset of CD4+ lymphocytes (29, 51).
HIV receptors and chemokines. Recognizing that the principal targets of HIV are CD4+ T cells and macrophages, in 1984 researchers established that the CD4 molecule was the primary receptor for virus entry into susceptible target cells. However, additional HIV receptors have been described including galactosylceramide on oligodendrocytes and Schwann cells in the brain and epithelial cells of the intestines. Immunoglobulin Fc receptors on neutrophils, monocytes, basophils, mast cells, eosinophils, platelets, and B lymphocytes also may facilitate binding of HIV. Antibodies made against various HIV antigens can bind to infectious virions or infected cells that, in turn, are bound by cellular Fc receptors. The bound complex can then be internalized by the cells and subsequently infect them independently of the CD4 receptor. There is current evidence indicating that CD4 alone is insufficient for optimal entry and fusion of HIV. This is based on the observation that murine cells genetically manipulated to express the human CD4 receptor are not permissive for HIV infection. Further, studies have shown that HIV grown in laboratory transformed T-cell lines could infect only primary T cells and could not infect monocytes and macrophages. These variants were designated T tropic. By contrast, primary HIV isolates could infect only monocytes and macrophages but not T-cell lines and hence were called macrophage (M) tropic. In addition there are some viruses that can infect both macrophages and T cells. These variations in cell tropism appear to be due to sequence differences in the V3 region of the envelope glycoprotein, gp120. When gp120 binds to CD4, changes occur in both molecules producing a new conformation that requires additional points of attachment for effective viral entry. Thus, supplementary, species-specific cell surface factors may be necessary for optimal virus fusion with the membrane. Such non-CD4 factors have been differentially named by various investigators as second receptors, coreceptors, fusion receptors, accessory receptors, or alternate receptors (35).
Recently, considerable interest has been directed to the identification and cloning of other putative coreceptors for HIV, yielding some surprises (1, 16, 48). A member of the seven transmembrane G-protein-coupled receptor family, termed leukocyte-derived seven transmembrane domain receptor (LESTER) or alternatively called fusin was found to act as a coreceptor for T-tropic HIV strains only. When fusin was introduced into HIV-resistant mouse cells expressing human CD4, they became readily susceptible to HIV infection. Recently, this coreceptor for T-tropic strains of HIV, fusin, was found to be identical to the chemokine receptor CXCR-4. The natural ligand for CXCR-4 is the chemokine, stromal cell-derived factor 1 (SDF-1). Chemokines are chemoattractant cytokines, many of which have long been known to play a role in mediating allergic reactions. SDF-1 can block the ability of CXCR-4 to serve as a coreceptor for T-tropic strains of HIV. Furthermore HIV-infected patients with SDF-1 gene variants were found to have a delay in the onset of AIDS (55). CXCR-4 was also shown to be the primary receptor for HIV-2. To reflect their coreceptor requirement, the T-cell tropic virus strains that require CXCR-4 have recently been renamed X4 viruses (6). The subsequent discovery of a coreceptor specific for M-tropic virus strains was not unexpected. This M-tropic HIV coreceptor was recognized to be the previously described chemokine receptor CCR5. Therefore, the M-tropic virus strains that require the CCR5 receptor for entry have been named R5 viruses (6). Other chemokine receptors, such as CCR2b and CCR3, also can serve as coreceptors for some HIV strains. The-chemokines RANTES (regulated upon activation, normal T-cell
expressed and secreted), and MIP-1
(macrophage inflammatory
protein-1) and MIP-1, are ligands for CCR5. CCR5 receptor binding
by these chemokines inhibited M-tropic virus infection of
CD4+ cells (17). RANTES is the most active
inhibitor of HIV replication. Moreover, the absence of CCR5 on a cell
has been associated with resistance to HIV infection. The role of CCR5
as coreceptor for HIV in vivo is supported further by a report of
resistance to HIV infection with R5 viruses by individuals who are
homozygous for a 32-bp CCR5 gene deletion (
32 CCR5) (19).
Independent confirmation of the role of chemokine receptors as
coreceptors for HIV derives from previous studies showing that HIV
replication in CD4+ cells could be suppressed by soluble
factors secreted from CD8+ cells. There is a current
controversy over whether these HIV suppressor factors are the
-chemokines RANTES, MIP-1, and MIP-1 or are a unique HIV
inhibitor (37). Although monocytes, B lymphocytes, mast
cells, and fibroblasts produce -chemokines in low amounts, activated
CD8+ cells are the most potent producers of them (18,
36). The role of the -chemokines in HIV infection has become
even more complicated in view of a recent report showing that they
stimulate HIV replication in macrophage cultures (48). While
there may be discrepancies between the various reports on the effect of -chemokines on HIV, it is evident that they have significant regulatory effects on virus replication. Further studies are necessary to elucidate the specific mechanisms underlying these observations. Perhaps they will lead to new therapeutic strategies using inexpensive synthetic blockers of the chemokine receptors or ways to regulate the
natural production of chemokines in vivo. Lastly, there is evidence for
another cellular HIV fusion domain that binds to envelope gp41
permitting entry of the viral core into host cells. A recent study also
identified proteins secreted by CD8+ from AIDS patients
that could block the infection of peripheral blood mononuclear cells by
both M-tropic and T-tropic isolates (42).
| |
DIAGNOSIS |
|---|
Serodiagnosis remains the primary method for detecting established HIV infections. Screening is performed by the enzyme-linked immunosorbent assay (ELISA). This technique depends upon antibodies from a serum sample to react with a crude extract of HIV particles. The ELISA technique has a sensitivity in the range of 93.4 to 99.8% and a specificity of 99.2 to 99.8%. If the initial ELISA result is positive the assay is repeated. After two successive positive ELISA results, the serum sample is then tested by the Western immunoblot technique. The Western blot technique detects antibodies to purified HIV proteins separated by electrophoresis; however, more recent versions of this method utilize recombinant HIV proteins. Specific antibodies binding to p24 plus at least one of the envelope proteins, gp120, gp41, or gp160, confirm seropositivity to HIV. Since the infected host takes at least 22 to 27 days to develop antibodies to HIV after infection, ELISA assays may not be able to detect acute HIV infection.
Other methods are also available for diagnosing HIV infections. The p24 antigen capture method is an immunoassay for the viral core protein. In vitro coculture of HIV-infected cells with susceptible cells also can be used to demonstrate infection. This method generally has been superseded by PCR. PCR is a powerful biological amplification technique that is capable of identifying very low copy numbers of proviral DNA in a complex mixture and exponentially expanding them to a level at which they can be detected readily. A variation on this technique can be used for detecting viral RNA, which is first reverse transcribed to DNA and then amplified by PCR. However the branched-DNA signal amplification assay is currently the method of choice to detect and quantitate viral RNA (viral load) in plasma. Viral load, rather than CD4 numbers, is now considered to be a better surrogate marker for prognosis of HIV infection (39).
Diagnosis of neonates born to HIV-seropositive mothers poses a special problem. As maternal immunoglobulin G (IgG) is transferred across the placenta during the last trimester of pregnancy, infants born to seropositive mothers also will be seropositive irrespective of their state of infection. Maternal antibodies can remain in the circulation of the infant for up to 1 year and consequently will confound serodiagnosis of the child. A positive assay for HIV p24 in the serum of a neonate is consistent with active infection. However the p24 antigen capture assay lacks sensitivity, and false-negative assay results are not uncommon. Thus the HIV DNA PCR assay is preferred for detecting viral genomes in neonates. IgA is not transplacentally transferred, and detection of IgA antibodies to HIV proteins in the serum of neonates and infants correlates with infection and seroconversion. Coculture of neonatal lymphocytes with susceptible target cells has been used for detection of active infections, but this method is no longer popular due the difficulties and biohazards of HIV culture.
Several commercial kits have been released for home testing of HIV infection. Considerable controversy has surrounded this issue. Clearly home testing is very convenient and appeals to privacy concerns. However, critics have argued that the emphasis on privacy may perpetuate the stigma of AIDS and that the quality of test-associated counseling may not be as good as personal counseling obtained directly from a health care professional. Another concern was for the high cost of home testing that may put it out of the reach of persons at greatest risk. Recently, one manufacturer withdrew its home testing kit because of a poor consumer response. As noted above, home testing which depends upon the assay of antibodies may not detect very early acute infections.
| |
CLINICAL MANIFESTATIONS |
|---|
Understandably it is difficult to identify patients acutely infected with HIV. However, the available information indicates that primary infection with HIV mimics more benign viral syndromes, particularly mononucleosis (43). During acute infection virus predominance may shift from the blood and localize in lymphoid tissues where extremely high rates of virus replication occur (44). While significant viral titers can be detected in circulation throughout the course of HIV infection in untreated individuals, increasing plasma viral titers during the late stages of disease may be an indicator of a poor prognosis. The clinical course of an HIV infection is depicted in Fig. 4. After primary infection there is a quiescent period during which the patient may be seronegative yet can be highly infectious. Ultimately antibodies are made to various HIV proteins and the patient becomes seropositive within 3 to 12 weeks after initial infection. However, it has been demonstrated that in one individual there was a lag of up to 39 months between initial infection and seroconversion. While this is an exception to the usual course of seroconversion, it demonstrates that it is possible for an individual to be infectious while remaining seronegative for a relatively long time.
Previously, the absolute CD4+ lymphocyte count was the primary marker for the clinical staging and prognosis of HIV infections (11). Currently viral load, as a function of plasma HIV-1 RNA levels (see above), is the preferred surrogate marker (39). The viral load at the time of seroconversion is not predictive of outcome, but the viral load after 3 to 6 months of infection is a good indicator of disease progression. Also, there is generally an inverse relationship between viral load and the absolute number of CD4+ lymphocytes (11). However, since some patients show increased CD4+ T-cell counts despite elevated viral load (34), measurement of both CD4 count and viral load is recommended to assess clinical status. During the asymptomatic phase of HIV infection, the total peripheral count tends to remain near normal. Paradoxically, the number of infected cells in the peripheral circulation is relatively low. This is due to a progressive homing of infected CD4+ cells to the lymph nodes, resulting in disruption of their germinal centers and disintegration of follicular dendritic cells. Within the lymph nodes infection may also spread to uninfected CD4+ cells, further increasing the local viral load. Thus the lymph nodes, where viral replication and numbers reach very high values, serve as major reservoirs for HIV.
As the infection progresses, persistent generalized lymphadenopathy may
develop. Concomitant with evidence of immunodeficiency, such as
delayed-type hypersensitivity skin test anergy, decreased in vitro
T-lymphocyte proliferative responses to mitogens and antigens, and/or
decreased NK cell activities (49), there may be an increase
in conditions that are suggestive of a defect in cell-mediated immunity
such as constitutional symptoms, bacillary angiomatosis, candidiasis,
thrombocytopenia, oral hairy leukoplakia, and peripheral neuropathy,
etc. With further disease progression there is an associated increase
in the incidence of opportunistic infections especially
Pneumocystis carinii pneumonitis. In addition, specific
malignancies, such as non-Hodgkin's lymphoma and Kaposi's sarcoma,
may develop. The latter is a malignant proliferation of vascular
endothelial cells which, prior to the HIV epidemic, occurred primarily
in men over 60 years old from the Mediterranean region. Kaposi's
sarcoma is associated with human herpesvirus (HHV) 8 infections and may
develop more readily in HIV-infected homosexual men than in other AIDS
risk groups (30). A list of AIDS-defining conditions is
presented in Table 2.
|
Encephalopathy is a serious complication of HIV infections. The AIDS dementia complex generally develops late in the course of infection in adults and then progresses unremittingly to death. It is characterized by cognitive, motor, and behavioral abnormalities. Biopsy and autopsy studies describe a wide range of cerebral lesions associated with AIDS encephalopathy ultimately producing cortical atrophy. Multinucleated giant cells are histopathologic correlates of the AIDS dementia complex, and vacuolar myelin damage may affect the hemispheric and interhemispheric white matter. Several virus-mediated neurological disorders have been reported in severely immunocompromised HIV-1-infected patients. Progressive multifocal leukoencephalopathy has been associated with the human polyoma JC virus. Primary central nervous system (CNS) lymphoma may develop secondary to infections with Epstein-Barr virus and/or Kaposi's sarcoma-associated herpesvirus, also known as HHV8. Other causes of HIV-1-associated CNS disease include (i) opportunistic infections particularly due to Toxoplasma gondii, herpesviruses, adenovirus, fungi, and mycobacteria and (ii) unusual primary malignancies, generally non-Hodgkin's lymphomas but non-lymphomatous neoplasms such as astrocytomas, oligodendrogliomas, and ependymomas have also been reported.
Pediatric considerations. Many of the general clinical manifestations described above are common to adults and children. However, there are several problems that are unique to the pediatric population. Like adults, children frequently develop pneumonitis caused by P. carinii. However they also are susceptible to an idiopathic lymphoid interstitial pneumonitis (LIP) that resembles P. carinii pneumonitis both clinically and radiographically. As therapy for these two entities is very different and often mutually exclusive, definitive diagnosis of LIP usually requires a lung biopsy. Therapy for Pneumocystis pneumonitis includes trimethoprim plus sulfamethaxazole or pentamidine, whereas idiopathic LIP is usually treated with systemic corticosteroids. Other clinical complications of HIV infections that are unique to children include failure to thrive, renal tubular acidosis, and a dysmorphology that is controversial.
In contrast to that in adults, encephalopathy in infants may be an early marker of AIDS. It usually presents as a failure to achieve normal, developmental, motor milestones. Early treatment with antiviral drugs such as zidovudine (ZDV) may completely reverse these symptoms, suggesting that the initial encephalopathy in infants may be due to transient neurotoxins or host factors such as cytokines. In support of this hypothesis is the observation that in spite of profound neurobehavioral symptoms, virus load within the brain generally is relatively low. Furthermore gp120 from the viral envelope was shown to be neurotoxic in vitro. With disease progression cortical atrophy and ventricular dilatation occurs, ultimately producing profound decreases in brain weight. Angiopathy with dystrophic calcification of blood vessels, particularly in the basal ganglia and pons, has been described.| |
THERAPY |
|---|
In addition to the primary therapy described below other medical management of HIV infection includes the use of antibiotics, antivirals, and antifungals for secondary or opportunistic infections, vaccination against other etiologic agents, prophylaxis of Pneumocystis pneumonitis, and psychological support. Although treatment of HIV-infected patients with recombinant (r)IL-2 or polyethylene glycol-modified rIL-2, alone or in combination with antiretroviral therapy, has produced some transient, beneficial changes in immunologic functions and CD4 counts, no substantial decrease in viral burden has been associated with IL-2 therapy (25).
Primary therapy for HIV infection involves combinations of various antiretroviral drugs. Early antiviral therapy of HIV infection is likely to be beneficial even in asymptomatic subjects. The mainstay of HIV treatment has been the use of RT inhibitors. RT inhibitors prevent the virus-derived enzyme, RT, from synthesizing viral DNA from the HIV genomic RNA template, thus preventing integration of subsequent viral cDNA into the host's genomic DNA. While RT inhibitors may hinder normal, cellular DNA synthesis, they are much more active against viral RT. ZDV (Retrovir), formerly called azidothymidine (AZT), is the prototypic RT inhibitor. It is an analog of thymidine, a natural precursor of DNA. Other nucleoside analogue RT inhibitors include didanosine (Videx), lamivudine (Epivir), stavudine (Zerit), and zalcitabine (HIVID). Efavirinz (Sustiva), delaviridine mesylate (Rescriptor) and nevirapine (Viramune) are nonnucleoside RT inhibitors (10).
Another class of antiretroviral drugs, the protease inhibitors such as indinavir (Crixivan), ritonavir (Norvir), nelfinavir (Viracept), and saquinavir (Fortovase and Invirase) are quite effective (10). These drugs block critical steps in virus assembly that are dependent upon proteolytic cleavage. The larger-molecular-weight gag-pol precursor gene product is post-translationally cleaved by viral proteases into the individual proteins that compose the nucleocapsid core (gag, p55, p24, p17, p15, p9, and p7) and the polymerases (pol) of HIV-1. However, the envelope precursor, gp160, is cleaved into gp120 and gp41 by host cell proteases. Synthetic inhibitors of the HIV and host cell proteases thus prevent the assembly of complete, infectious virions resulting in morphologically abnormal, noninfectious particles. Additions to the pharmacopoeia of antiviral drugs occur quite frequently.
Single-drug treatment or monotherapy against HIV infection is not effective because of the rapid emergence of drug-resistant viral mutants. Multidrug, combination therapy currently is the strategy for HIV management. However, there is no definitive evidence that multidrug therapy can completely eliminate the virus. While there have been many observations and reports of treated patients who have dropped their viral loads below the level of detection, their long-term prognosis remains guarded (3). Regarding initial therapy, two major factors must be considered: the viral load and the commitment of the patient to rigid adherence to lifelong treatment. Initiation of therapy should be considered for patients with HIV RNA levels greater than 5,000 to 10,000 copies/ml regardless of CD4 count. It is currently recommended that initial treatment consist of a three-drug regimen including two different nucleoside analog RT inhibitors (NRTI) plus a potent protease inhibitor (10). A combination of two different NRTIs plus a nonnucleoside RT inhibitor (NNTI) is an acceptable alternative. Increasing HIV RNA levels suggest treatment failure and are an indication for changing therapy. Other reasons for considering changing therapy include toxicity, intolerance, and noncompliance. When switching therapy at least two and preferably all three drugs should be changed. Single drug changes are strongly discouraged. A wide range of alternative combinations have been proposed (10). Limited CD4+ T-cell increases have been reported for the highly active antiretroviral therapy (HAART) in early HIV-1 infections (23). Although HAART regimens are generally well tolerated by HIV-infected patients, several adverse effects have been described including altered body habitus, hypoglycemia, and hyperlipidemia.
Pregnancy in an HIV-infected woman poses a unique therapeutic problem as the needs of both the fetus and the mother must be considered in planning therapy. The rate of vertical transmission of HIV from an infected mother to her child is approximately 20% in the untreated state in developed countries. A National Institutes of Health-supported clinical trial (ACTG 076) demonstrated that treatment of HIV-infected, pregnant women with ZDV commencing at 14 weeks of gestation can significantly reduce the rate of vertical transmission to the infant to about 8%. Only relatively short-term safety data is available from this trial. The sole form of infant toxicity observed was a mild, transient anemia that resolved by postnatal week 12. No congenital anomalies were observed. Regarding other retrovirals, there have been reports of premature deliveries by pregnant women treated with drug combinations including indinavir or ritonavir. However, it is not possible to determine whether this specifically was due to the protease inhibitors or to the combination used. Because of the lack of sufficient data, caution should be exercised when considering protease inhibitors during pregnancy. In any treatment plan it is essential that the risks and benefits to both mother and fetus are explained so that an informed decision can be made.
In children, treatment with intravenous IG (IVIG) was shown to reduce the morbidity but not the overall mortality of HIV infections by decreasing the severity and frequency of opportunistic infections (40). However, this benefit was limited to a subgroup of children who were not receiving trimethoprim-sulfamethoxazole for Pneumocystis prophylaxis (50). Recently, a clinical trial of IVIG in HIV-infected adults also showed that the frequency of serious infections and concomitant hospitalizations were significantly decreased. However, while IVIG was shown to reduce the incidence of secondary infections associated with HIV-1 disease in both adults and children (56), further studies are needed to assess the possibility of antibody-mediated enhancement of HIV-1 infections via Fc and complement receptors on the surface of cells. This could be a mechanism for infection of other target cells in addition to CD4+ cells.
| |
PREVENTION |
|---|
As HIV infection is an STD, a vigorous educational program to promote safe sex practices is paramount to reducing transmission of HIV (4). Barrier protection with latex condoms is helpful. There has been speculation that the spermicide nonoxyl 9 may have anti-HIV activity, but this has not been substantiated in a controlled clinical trial. Unprotected, receptive anal intercourse among homosexual men is a high-risk activity. Screening of blood donors for HIV antibodies and donated blood and derivative products for the p24 core antigen has improved the safety of the blood supply. There is a "window period" of approximately 22 to 25 days after initial infection before detectable seroconversion occurs. The p24 antigen capture assay was proposed to shorten this window period by 5 to 10 days. However, it lacks sensitivity to low levels of antigen and antigenemia often is transient. When antibodies to p24 are present, they can mask detection of antigen by forming immune complexes. The p24 antigen assay was unable to detect up to 75% of seronegative blood donors who were infected (26), and its mandated use adds a major cost to processing donated blood. Thus, additional methods such as heat and detergent treatment, increased purification, and the use of recombinant materials (e.g., rFactor VIII), etc. are needed to make blood products safer. HIV infection among intravenous drug users and their sexual partners has been increasing steadily. Although politically controversial, there is evidence that the ready availability of sterile hypodermic needles and syringes can reduce HIV transmission. This has been attempted through exchange programs or by eliminating the need for prescriptions to purchase syringes and hypodermic needles from pharmacies.
Clearly health care workers are at increased risk of exposure to HIV. Because of this occupational hazard, public health authorities have implemented the practice of universal body fluid precautions. Thus, all body fluids from all patients should be handled as if they contained infectious virus. Skin with open lesions and mucous membranes are particularly vulnerable. Hence the use of latex gloves and face shields is strongly recommended to reduce the risk of occupational exposure. Recapping of hypodermic needles presents a high risk for injury and this habit must cease. All contaminated needles and sharp instruments should be placed directly into a secure, closed container for subsequent sterilization.
An earlier epidemiological investigation of health care workers by the CDC demonstrated that the risk of seroconversion after percutaneous exposure (e.g., needle stick or laceration) to a known infected source was about 0.5%. The average risk of HIV infection from all types of exposure to infected blood is only 0.3%. Even though these are remarkably low rates, the consequences of HIV infection are so serious that prevention is the best option. Several studies have demonstrated a potential benefit from postexposure chemoprophylaxis of HIV infections (45). Thus, the CDC developed guidelines for a 4-week course of chemoprophylaxis in the event of an occupational exposure to HIV. Prophylaxis ranges from single-drug treatment with ZDV alone to a three-drug regimen in cases of exposure with the highest risk. Exposed individuals should be tested for seroconversion at 6 and 12 weeks and at 6 months and should be counseled about the possibility of secondary transmission. If chemoprophylaxis is instituted, persons should be evaluated for drug toxicity by monitoring complete blood counts and by performing renal and hepatic functional assays. Prophylaxis of opportunistic infections should also be considered along with antiretroviral prophylaxis for certain high-risk groups.
Vaccines. In any virus infection, the guiding principle for an effective vaccine strategy derives from the natural immunity which is part of the recovery process. In addition to stimulating protective antibodies against HIV the ideal vaccine should also induce specific cytotoxic T lymphocytes against HIV-infected cells and activate nonspecific NK cells. In experimental systems, HIV can induce vigorous humoral and cell-mediated immune responses that can effectively neutralize the virus and lyse infected cells. However, in the clinical situation, host immune responses do not seem adequate to eliminate HIV infections. This places HIV in the category of viruses against which an effective vaccine has yet to be developed (21). Vaccines have been the most effective defense against other viral diseases such as polio and smallpox. Development of a potent vaccine against HIV has been complicated by a number of factors including: (i) the genomic variability of the virus, (ii) a lack of good animal models, (iii) a lack of satisfactory surrogate markers of protective immunity, (iv) the intracellular mode of HIV transmission, and (v) the persistent nature of infection. Since 80% of HIV infections occurs sexually, a good vaccine should stimulate mucosal immunity particularly in the reproductive tract. Use of live, attenuated or whole, inactivated HIV as a vaccine has advantages such as easy preparation and potential induction of long-term, natural immunity. However some concerns such as variability of virus strains, contamination of vaccine with host cell proteins, and safety in immunodeficient patients remain to be assessed. Several candidate HIV vaccines are composed of synthetic, recombinant, or highly purified subunit epitopes spanning various regions of the HIV proteins gp120, gp41, Tat, Rev, and Nef. Subunit antigens are considered to be safe in comparison with killed whole or live-attenuated virus, but subunit vaccines are generally less immunogenic. Neutralizing antibodies have been detected against a specific epitope of gp120, the V3 loop, and this region has attracted considerable attention as a vaccine candidate. Currently various adjuvants, such as detoxified lipid A, adjuvant emulsions, liposomes, biodegradable microspheres, muramyl peptides, and saponin, are being evaluated for their ability to increase immune responses to HIV vaccines. The recent discovery of the X-ray crystallographic structure of gp120, the subsequent revelation of the gp120-CD4 interface, and identification of the conserved site for the chemokine receptor (33) may provide critically needed information to develop an effective and safe HIV vaccine.
While the search for an effective HIV vaccine remains elusive, there are some unique clinical observations that suggest there are intrinsic host protective mechanisms against the virus that can be upregulated by vaccination. Individuals who are seropositive for HIV but show no evidence of viral genome have been reported, suggesting the possibility of a spontaneous remission. Also there is a cohort of African prostitutes who are evidently at high risk but have not seroconverted nor do they harbor virus genome. All of these observations are encouraging and support the continuation of efforts to develop an HIV vaccine.| |
GENE THERAPY |
|---|
In spite of the advances described above, a definitive cure for HIV infection remains elusive (46). This is partly due to the unique life cycle of the virus as well as its plasticity and antigenic variability. Genetic manipulation of somatic cells has recently been proposed for prophylaxis and therapy against a variety of infectious diseases including HIV. This involves the stable insertion of "resistance genes," also called intracellular immunization, into HIV-susceptible cells to render them resistant to infection. Further, the ectopic expression of genes encoding specific viral antigens that evoke antiviral immune responses is also currently being evaluated. These approaches include the use of modified transdominant HIV proteins, RNA decoys, antisense RNA, ribozymes, and cellular proteins such as soluble CD4. Plasmids containing "naked" DNA encoding various HIV-1 genes have recently been injected into animals, including nonhuman primates, and human volunteers as potential vaccines. Thus, the HIV-1 genes are expressed in vivo in the absence of infectious virus and the resultant gene products may induce immune responses by the host. Whether these new methods can protect against infection with HIV-1 remains to be determined. Nevertheless they are promising and ongoing research may yield a long-awaited breakthrough.
| |
ACKNOWLEDGMENTS |
|---|
Our research described herein was supported by NIH grants RO1 MH47225, RO3 DA11119, and R01 DA010632-01A1; the Margaret Duffy and Robert Cameron Troup Memorial Fund for Cancer Research of the Buffalo General Hospital; and the Theodore T. Jacobs, M.D., Endowment for Immunology Research of the Buffalo General Foundation.
| |
FOOTNOTES |
|---|
* Corresponding author. Mailing address: Division of Allergy, Immunology, & Rheumatology, Buffalo General Hospital, 100 High St., Buffalo, NY 14203. Phone: (716) 859-2985. Fax: (716) 859-2999. E-mail: sasimmun{at}acsu.buffalo.edu.
| |
REFERENCES |
|---|
|
Top
Introduction
References
|
|---|
| 1. | Alkhatib, G., C. Combadiere, C. Broder, Y. Feng, P. E. Kennedy, P. M. Murphy, and E. A. Berger. 1996. CC CKR5: a RANTES, MIP-1a, MIP-b receptor as a fusion cofactor for macrophage-tropic HIV-1. Science 272:1955-1958[Abstract]. |
| 1a. | Anonymous. 1998. AIDS epidemic update. Joint United Nations programme on HIV/AIDS. Geneva, Switzerland . |
| 2. |
Balter, M.
1997.
How does HIV overcome the body's T cell bodyguards?
Science
278:1399-1400 |
| 3. | Bartlett, G. 1997. Protease inhibitors, a new class of drugs against human immunodeficiency virus. Human herpesvirus-8 and hepatitis G, newly identified causes of human disease. The role of infectious agents in "noninfectious" disease. JAMA 277:1865-1866[Medline]. |
| 4. | Beekmann, S. E., and D. K. Henderson. 1995. HIV infection in healthcare workers: risk for infection and methods of prevention. Semin. Dermatol. 14:212-218[Medline]. |
| 5. | Benito, J. M., J. M. Zabay, J. Gil, M. Bermejo, A. Escudero, E. Sanchez, and E. Fernandez-Cruz. 1997. Quantitative alterations of the functionally distinct subsets of CD4 and CD8 T lymphocytes in asymptomatic HIV infection: changes in the expression of CD45RO, CD45RA, CD46, CD38, HLA-DR, and CD25 antigens. J. Acquired Immune Defic. Syndr. Hum. Retrovirol. 14:128-135[Medline]. |
| 6. | Berger, E. A., R. W. Doms, E.-M. Feryo, et al. 1998. A new classification for HIV-1. Nature 391:240[Medline]. |
| 7. | Black, R. F. 1996. Transmission of HIV-1 in the breast-feeding process. J. Am. Dietetic Assoc. 96:267-274[Medline]. |
| 8. | Boudet, F., H. Lecoeur, and M. L. Gougeon. 1996. Apoptosis associated with ex vivo down-regulation of Bcl-2 and up-regulation of Fas in potential cytotoxic CD8+ T lymphocytes during HIV infection. J. Immunol. 156:2282-2293[Abstract]. |
| 9. | Bruunsgaard, H., C. Pedersen, E. Scheibel, and B. K. Pedersen. 1995. Increase in percentage of CD45RO+/CD8+ cells is associated with previous severe primary HIV infection. J. Acquired Immune Defic. Syndr. Hum. Retrovirol. 10:107-114[Medline]. |
| 10. | Carpenter, C. C., M. A. Fischl, S. M. Hammer, M. S. Hirsch, D. M. Jacobsen, D. A. Katzenstein, J. S. Montaner, et al. 1996. Antiretroviral therapy for HIV infection in 1996. Recommendations of an international panel. International AIDS Society-USA. JAMA 276:146-154[Abstract]. |
| 11. | Centers for Disease Control. 1992. 1993 revised classification system for HIV infection and expanded surveillance case definition for AIDS among adolescents and adults. Morbid. Mortal. Weekly Rep. 41:961-962. |
| 12. | Centers for Disease Control and Prevention. 1998. Notifiable diseases/deaths in selected cities. Morbid. Mortal. Weekly Rep. 47:1101-1116. |
| 12a. | Centers for Disease Control and Prevention. 1998. HIV/AIDS surveillance report, vol. 10. , p. 1-40. Centers for Disease Control and Prevention, Atlanta, Ga. |
| 13. | Chaudry, M. N., and D. H. Shepp. 1997. Antiretroviral agents. Current usage. Dermatol. Clinics 15:319-329[Medline]. |
| 14. | Chen, I. S., and I. D. Rosenblatt. 1991. Human T-cell leukemia virus type II, p. 21-33. In R. C. Gallo, and G. Jay (ed.), The human retroviruses. Academic Press, San Diego, Calif. |
| 15. | Clerici, M., and G. M. Shearer. 1992. Th2 switch is a critical step in the etiology of HIV infection. Immunol. Today 14:107-111. |
| 16. |
Cocchi, F.,
A. J. DeVico,
A. Grazino-Demo,
S. K. Arya,
R. C. Gallo, and P. Lusso.
1995.
Identification of RANTES, MIP-1 and MIP- as the major HIV suppressive factors produced by CD8+ T cell.
Science
270:1811-1815 |
| 17. |
Cohn, J.
1997.
Exploiting the HIV-chemokine nexus.
Science
275:1261-1262 |
| 18. | Conlon, K., A. Lloyd, U. Chattopadhyay, N. Lukacs, S. Kunkel, T. Schall, D. Taub, C. Morimoto, J. Osborne, and J. Oppenheim. 1995. CD8+ and CD45RA+ human peripheral blood lymphocytes are potent sources of macrophage inflammatory protein 1 alpha, interleukin-8 and RANTES. Eur. J. Immunol. 25:751-756[Medline]. |
| 19. |
Dean, M.,
M. Carrington,
C. Winkler,
G. A. Huttley,
M. W. Smith, et al.
1996.
Genetic restriction of HIV-1 infection and progression to AIDS by a deletion allele of the CKR-5 structural gene.
Science
273:1856-1862 |
| 20. | Doran, C. M. 1997. New approaches to using antiretroviral therapy for the management of HIV infection. Ann. Pharmacother. 31:228-236[Abstract]. |
| 21. | Esparaza, J., S. Osmanov, and W. L. Heyward. 1995. HIV preventive vaccines. Progress to date. Drugs 50:792-804[Medline]. |
| 22. | Feingberg, M. B., and A. R. McLean. 1997. AIDS: decline and fall of immune surveillance? Curr. Biol. 7:R136-R140[Medline]. |
| 23. | Fluery, S., R. J. DeBaer, G. Rizzardi, et al. 1998. Limited CD4+ T cell renewal in early HIV-I infection: effect of highly active antiretroviral therapy. Nat. Med. 4:794-801[Medline]. |
| 24. | Fouchier, R. A., L. Meyaard, M. Brouwer, E. Hovenkamp, and H. Schuitemaker. 1996. Broader tropism and higher cytopathogenicity for CD4+ T cells of a syncytium-inducing compared to a non-syncytium-inducing HIV-1 isolate as a mechanism for accelerated CD4+ T cell decline in vivo. Virology 219:87-95[Medline]. |
| 25. | Fyfe, G. A., and H. C. Lane. 1996. Biologic response modifiers (interleukins and interferons), p. 493-511. In S. Gupta (ed.), Immunology of HIV infection. Plenum Press, New York, N.Y. |
| 26. | Gilmore, N. 1996. Blood and blood product safety, p. 287-301. In J. Mann, and D. Tarantola (ed.), AIDS In the world. Oxford University Press, Oxford, United Kingdom. |
| 27. |
Gouen, M. L., and L. Montagnier.
1993.
Apoptosis in AIDS.
Science
260:1269-1270 |
| 28. | Haseltine, W. A., and F. Wong-Staal. 1988. The molecular biology of the AIDS virus. Sci. Am. 259:52-60[Medline]. |
| 29. | Helbert, M. R., J. Walter, J. L'Age, and P. C. Beverley. 1997. HIV infection of CD45RA+ and CD45RO+ CD4+ T cells. Clin. Exp. Immunol. 107:300-305[Medline]. |
| 30. | Kimura, S. 1997. Virus-related neurological disorders complicating in compromised hosts. Nippon Rinsho Jpn. J. Clin. Med. 55:949-953. |
| 31. | Klatzman, D., E. Champagne, and E. Chamaret. 1984. T-lymphocyte T4 molecule behaves as the receptor for human retrovirus LAV. Nature 312:767-768[Medline]. |
| 32. | Koito, A., L. Stamatatos, and C. Cheng-Mayer. 1995. Small amino acid sequence changes within the V2 domain can affect the function of a T-cell line-tropic human immunodeficiency virus type I envelop gp 120. Virology 206:878-884[Medline]. |
| 33. | Kwong, P. B., R. Wyatt, J. Robinson, R. W. Sweet, J. Sordroski, and A. W. Hendrickson. 1998. Structure of an HIV-gp 120 envelop glycoprotein in complex with the CD4 receptor and a neutralizing human antibody. Nature 393:648-657[Medline]. |
| 34. |
Levitz, S. M.
1998.
Improvement in CD4+ cell counts despite persistently detectable HIV load.
N. Engl. J. Med.
338:1074-1075 |
| 35. |
Levy, J. A.
1996.
Infection by human immunodeficiency virus CD4 is not enough.
N. Engl. J. Med.
335:1528-1530 |
| 36. | Liles, W. C., and W. C. Van Voorhis. 1995. Nomenclature and biologic significance of cytokines involved in inflammation and the host immune response. J. Infect. Dis. 172:1573-1580[Medline]. |
| 37. | Mackenwicz, C., and J. A. Levy. 1992. CD8+ cell anti-HIV activity: nonlytic suppression of virus replication. AIDS Res. Hum. Retrovirus 8:1039-1050[Medline]. |
| 38. |
Markovitz, D. M.
1993.
Infection with the human immunodeficiency virus type-2.
Ann. Intern. Med.
118:211-218 |
| 39. | Mellors, J. W., C. R. Rinaldo, Jr., P. Gupta, R. M. White, J. A. Todd, and L. A. Kingsley. 1996. Prognosis in HIV-1 infection predicted by the quantity of virus in plasma. Science 272:1167-1170[Abstract]. |
| 40. | Mofenson, L. M., J. Moye, Jr., J. Bethel, R. Hirschorn, C. Jordan, and R. Nugent. 1992. Prophylactic intravenous immunoglobulin in HIV-infected children with CD+ counts of 0.20 × 109/L or more. Effect on viral, opportunistic, and bacterial infections. The National Institute of Child Health and Human Development Intravenous Immunoglobulin Clinical Trial Study Group. JAMA 268:483-488[Abstract]. |
| 41. | Muro-Cacho, C. A., G. Pantaleo, and A. S. Fauci. 1995. Analysis of apoptosis in lymph nodes of HIV-infected persons. Intensity of apoptosis correlates with the general state of activation of the lymphoid tissue and not with stage of disease or viral burden. J. Immunol. 154:5555-5566[Abstract]. |
| 42. |
Pal, R.,
A. Garzino-Demo,
P. D. Markham,
J. Burns,
M. Brown,
R. C. Gallo, and A. L. Devico.
1997.
Inhibition of HIV-I infection by the -chemokine MDC.
Science
278:695-698 |
| 43. |
Pantaleo, G.,
C. Graziosi, and A. S. Fauci.
1993.
The immunopathogenesis of human immunodeficiency virus infection.
N. Engl. J. Med.
328:327-335 |
| 44. | Perelson, A. S., A. U. Neumann, M. Markowitz, J. M. Leonard, and D. D. Ho. 1996. HIV-1 dynamics in vivo: virion clearance rate, infected cell life span, and viral generation time. Science 271:1583-1586. |
| 45. | Perlmutter, B. L., and B. R. Harris. 1997. New recommendations for prophylaxis after HIV exposure. Am. Family Phys. 55:507-517[Medline]. |
| 46. | Poeschla, Y. M., and F. Wong-Stall. 1994. Progress towards gene therapy of HIV infection. Gene Ther. 1:13-26[Medline]. (Review.) |
| 47. | Ratner, L. 1996. Genetic organization of HIV, p. 3-22. In S. Gupta (ed.), Immunology of HIV Infection. Plenum Press, New York, N.Y. |
| 48. | Schmidtmayerova, H., B. Sherry, and M. Bukrinsky. 1996. Chemokines and HIV replication. Nature 382:767[Medline]. |
| 49. | Schnittman, A. M., and A. S. Fauci. 1994. Human immunodeficiency virus and acquired immunodeficiency syndrome: an update. Adv. Intern. Med. 39:305-354[Medline]. |
| 50. | Shioda, T., J. A. Levy, and C. Chang-Mayer. 1991. Macrophage and T cell-line tropisms of HIV-I are determined by specific regions of the envelop gp 120 gene. Nature 349:167-169[Medline]. |
| 51. |
Spector, S. A.,
R. D. Gelber,
N. McGrath,
D. Wara, and A. Barzilai.
1994.
A controlled trial of intravenous immune globulin for the prevention of serious bacterial infections in children receiving zidovudine for advanced human immunodeficiency virus infection.
N. Engl. J. Med.
331:1181-1187 |
| 52. | Spina, C. A., H. E. Prince, and D. D. Richman. 1997. Preferential replication of HIV-1 in the CD45RO memory cell subset of primary CD4 lymphocytes in vitro. J. Clin. Investig. 99:1774-1785[Medline]. |
| 53. |
Travers, K.,
S. Mboup,
R. Marlink,
A. Gueye-Nidaye,
T. Siby,
I. Thior,
I. Traore,
A. Dieng-Sarr,
J. L. Sankale,
C. Mullins, et al.
1995.
Natural protection against HIV-1 infection provided by HIV-2.
Science
268:1612-1615 |
| 54. | Van de Perre, P., P. Lepage, J. Homsy, and F. Davis. 1992. Mother-to-infant transmission of human immunodeficiency virus by breast milk: presumed innocent or presumed guilty? Clin. Infect. Dis. 15:502-507[Medline]. |
| 55. |
Winkler, C.,
W. Modi,
M. O. Smith, et al.
1998.
Genetic restriction of AIDS pathogenesis by an SOFI chemokine gene variant.
Science
279:389-393 |
| 56. | Yap, P. L. 1994. Does intravenous immune globulin have a role in HIV-infected patients? Clin. Exp. Immunol. 1:59-67. |
This article has been cited by other articles:
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
