Identifying the Target Cell in Primary Simian Immunodeficiency Virus (SIV) Infection: Highly Activated Memory CD4+ T Cells Are Rapidly Eliminated in Early SIV Infection In Vivo

doi:10.1128/JVI.74.1.57-64.2000

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Journal of Virology, January 2000, p. 57-64, Vol. 74, No. 1
0022-538X/0/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Identifying the Target Cell in Primary Simian Immunodeficiency Virus (SIV) Infection: Highly Activated Memory CD4⁺ T Cells Are Rapidly Eliminated in Early SIV Infection In Vivo

Ronald S. Veazey,^* Irene C. Tham, Keith G. Mansfield, MaryAnn DeMaria, Amy E. Forand, Daniel E. Shvetz, Laura V. Chalifoux, Prabhat K. Sehgal, and Andrew A. Lackner

New England Regional Primate Research Center, Harvard Medical School, Southborough, Massachusetts 01772

Received 3 May 1999/Accepted 21 September 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

It has recently been shown that rapid and profound CD4⁺ T-cell depletion occurs almost exclusively within the intestinal tractof simian immunodeficiency virus (SIV)-infected macaques withindays of infection. Here we demonstrate (by three- and four-colorflow cytometry) that this depletion is specific to a definablesubset of CD4⁺ T cells, namely, those having both a highly and/or acutely activated(CD69⁺ CD38⁺ HLA-DR⁺) and memory (CD45RA Leu8) phenotype. Moreover, we demonstrate that this subset of helperT cells is found primarily within the intestinal lamina propria.Viral tropism for this particular cell type (which has been previouslysuggested by various studies in vitro) could explain why profoundCD4⁺ T-cell depletion occurs in the intestine and not in peripherallymphoid tissues in early SIV infection. Furthermore, we demonstratethat an acute loss of this specific subset of activated memoryCD4⁺ T cells may also be detected in peripheral blood and lymph nodesin early SIV infection. However, since this particular cell typeis present in such small numbers in circulation, its loss doesnot significantly affect total CD4⁺ T cell counts. This finding suggests that SIV and, presumably,human immunodeficiency virus specifically infect, replicate in,and eliminate definable subsets of CD4⁺ T cells invivo.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Although human immunodeficiency virus (HIV) infection is generally associated with a prolonged period of clinical latency,increasing evidence points to the importance of early events fordetermining the outcome of HIV infection (25, 34). Unfortunately,early (first month) events in the pathogenesis of HIV infectionare poorly characterized, mainly due to the difficulty in obtainingappropriate samples from humans with primary infection. Furthermore,examination of peripheral lymph nodes and blood provides a limitedview of the immunopathologic processes that are occurring in earlyinfection. For example, it has recently been shown that simianimmunodeficiency virus (SIV) infection causes profound loss ofCD4⁺ T cells from within the intestinal immune system (which is thelargest immunologic organ in the body) long before any significantT-cell alterations occur in peripheral lymph nodes or blood (24,48, 53). Although mounting evidence also implicates the intestinaltract as a major target organ in early HIV infection (12, 27,46, 53, 54), it is difficult to adequately examine the intestinaltracts of humans with early HIV infection. Fortunately, observationsof viral loads and distribution of SIV in lymphoid tissues ofacutely infected macaques have been validated as an excellentmodel of the effects of HIV in human tissues (38). Moreover,it has been demonstrated that the intestinal T-cell compartmentsof rhesus macaques are more similar to those of humans than anyother laboratory animal (55). Thus, characterizing the effectsof SIV infection on gut-associated lymphoid tissues in the SIV-rhesusmodel is highly relevant to HIV infection inhumans.

To explain the increased tissue viral loads and the rapidity of CD4⁺ T-cell losses in the intestine, we hypothesized that SIV optimallyreplicates within CD4⁺ T cells having an activated, memory immunophenotype, which arepresent in abundance in the intestinal tract. In vitro experimentswith HIV have demonstrated that peripheral blood CD4⁺ T cells may remain latently infected with provirus indefinitely.However, appropriate activation of these cells consistently resultsin productive viral replication and cell lysis (16, 19). Severalother in vitro studies have confirmed that optimal viral replicationoccurs only in CD4⁺ T cells having an activated and/or memory phenotype (8, 10,11, 31, 33, 36, 47, 49, 52, 58). Moreover, activatedmemory CD4⁺ T cells have been shown to express high levels of CCR5, whichis a major coreceptor for both SIV and HIV (7, 17). Therefore,it was reasonable to hypothesize that the reason intestinal laminapropria CD4⁺ T cells are eliminated first is that they are predominantly activatedand/or memory cells. To test this hypothesis, four-color flowcytometry was performed on lymphocytes isolated from both theintestinal epithelium and lamina propria of the jejunum, ileum,and colon and compared to results for lymphocytes from peripheraland mesenteric lymph nodes, spleen, and blood. Lymphocyte phenotypeswere compared by using a panel of monoclonal antibodies designedto distinguish naive from memory T cells, as well as to categorizethe expression of an array of markers associated with cellularactivation on well-defined T-cell subsets (Table 1). Since intestinallamina propria CD4⁺ T cells are essentially depleted within the first 2 weeks ofSIV infection (24, 48, 53), emphasis was placed on phenotypingpercentages and numbers of intestinal lamina propria CD4⁺ T cells in uninfected, normal rhesus macaques and in those withvery early SIV infection (up to 2 weeks postinoculation [p.i.]).SIV-infected animals in the early stages of infection were alsocompared to those in the terminal stage of disease (AIDS).

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TABLE 1. Cell surface marker expression examined on lymphocytes by four-color flow cytometry

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Examination of T-cell subsets and activation state by flow cytometry. To assess lymphocyte activation and distinguish naive from memory T cells, a variety of antibodies against cell surface markerswere used in various combinations, based on current knowledgeof T-cell activation and memory (Table 1). Activation markersincluded CD69, a cell surface antigen expressed very early inT-cell activation (59), CD28, a costimulatory molecule importantin T-cell activation and cytokine regulation (6, 15, 26,28, 51), CD38, a transmembrane glycoprotein thought to beinvolved in T-cell signaling, activation, and adhesion (2,32, 42), and HLA-DR (a major histocompatibility complex typeII [MHC II] molecule), which is also upregulated on activatedlymphocytes. To distinguish naive from memory CD4⁺ T cells, expression of CD45RA and CD62L (L-selectin) was examined.Although the concept of naive and memory T cells is continuouslybeing revised (reviewed by Bell et al. [3]), it is currentlythought that CD4⁺ T lymphocytes that have not previously (or at least not recently)encountered their T-cell receptor (TCR)-specific antigen expressthe CD45RA isoform of the common leukocyte antigen, CD45. Lymphocytesthat have previously encountered antigen are known to expressthe CD45RO isoform (3). Unfortunately, existing anti-humanCD45RO monoclonal antibodies do not cross-react in the rhesusmacaque, and so memory and naive CD4⁺ T lymphocytes are defined in this report as either CD45RA⁺ (naive) or CD45RA (memory). Since there is a transient switching period in whichcells may express both isoforms of CD45, antibodies against CD62Lwere simultaneously used to help distinguish truly naive (CD45RA⁺ CD62L⁺) from memory (CD45RA CD62L^+/) lymphocytes in peripheral blood and lymph nodes, using previouslydescribed methodology (40, 43). However, it is important tonote that CD62L (a peripheral lymph node homing receptor) is notusually expressed on intestinal lamina propria lymphocytes (LPL)(4). Since CD62L is shed rapidly upon lymphocyte activation(51), this may be another reflection of the highly activatedstate of intestinal LPL. Although CD62L plays a minor role intrafficking of naive lymphocytes to the intestinal inductive lymphoidtissues (Peyer's patches and lymphoid follicles), other homingmolecules (such as $alpha$ 4 $beta$ 7 and $alpha$ E $beta$ 7) primarily govern the homingof lymphocytes to the diffuse effector lymphoid tissues (laminapropria) of the intestine (9). Therefore, while CD62L is particularlyuseful in defining resting naive lymphocytes (CD62L⁺ CD45RA⁺) in peripheral lymphoid tissues, it may not be as useful in discriminatingnaive and memory cells in the intestine. For these reasons, naiveand memory CD4⁺ T cells in the intestine were defined primarily on the basisof CD45RA expression. With this rationale, activated memory CD4⁺ T cells should be both CD45RA and CD62L negative, regardlessof the tissueexamined.

Animals and virus. A total of 39 rhesus macaques were examined in this study. Of these, 29 were sacrificed by barbiturate overdose, and lymphoidtissues were harvested at necropsy. An additional 10 animals werefollowed prospectively, with sequential intestinal lymphoid tissuescollected by biopsy in three of these animals. Of the 29 animalsfrom which tissues were collected at necropsy, 10 were uninfectedcontrols, 15 were juvenile (1- to 2-year-old) males in the acutestage of infection, and 4 were adults with terminal AIDS. Of thesacrificed controls, seven were adult (5- to 20-year-old) females,two were adult males, and one was a 2-year-old juvenile. The 15animals in the acute stage of infection were juveniles infectedwith equal doses (50 ng of p27) of SIVmac239 or SIVmac251 intravenously.We have previously shown that these two viruses have identicaleffects on intestinal lymphocytes (53) and virtually identicalcourses of disease in macaques (56). Therefore animals infectedwith these viruses were grouped together. Of the 15 acutely infectedanimals, 5 were sacrificed and examined at 7 days p.i., 4 weresacrificed and examined at 14 days p.i., and an additional 6 animalsin groups of two were sacrificed and examined at 3, 21, and 50days p.i. Data on the intestinal CD4 depletion from some of theacutely infected animals have previously been reported (53).The four animals sacrificed in the terminal stages of infection(AIDS) had been inoculated with similar doses of either SIVmac239or SIVmac251 at least 1 year prior tosacrifice.

To determine whether age differences could account for the differences observed between the control and uninfected animals,a prospective analysis was performed on an additional 10 juvenilemacaques intravenously infected with SIVmac251 (50 ng of p27).From these, peripheral blood was examined before infection andat 7, 14, 21, and 30 days following infection. In addition, sequentialendoscope-guided intestinal pinch biopsies of duodenum and colonwere obtained from three of these animals prior to infection andat 7, 14, 21, and 35 days p.i. to assess longitudinal changesin intestinal lymphocytesubsets.

Isolation of lymphocytes and flow cytometry. Segments of intestine 6 to 8 cm long from jejunum, ileum, and colon were collected from the 29 animals that were killed, andlymphocytes were separately isolated from the intestinal epithelium(intraepithelial lymphocytes [IEL]) and lamina propria (LPL) fromeach intestinal segment as previously described (53, 55).Sections of jejunum were consistently taken between 30 and 40cm distal to the pylorus (proximal jejunum) to obtain representativeLPL and IEL (which comprise the effector arm of the intestinalimmune system) with minimal contamination from organized lymphoidtissues (the inductive arm of the intestinal immune system). Incontrast, cells obtained from sections of ileum and colon weremore likely to contain lymphocytes from both effector sites (LPLand IEL) and inductive sites (Peyer's patches and solitary lymphoidfollicles), the latter of which contain higher proportions ofnaive restinglymphocytes.

Endoscope-guided pinch biopsies from the proximal jejunum and distal colon were collected from three juvenile macaques atmultiple time points. These biopsies were processed and examinedseparately, but no attempt was made to separate IEL from LPL inthese samples. Since IEL are essentially all CD8⁺ T cells, this resulted in slightly lower percentages of CD4⁺ T cells in these samples, but since CD4⁺ T cells are mostly found in the lamina propria (55), no differencesin phenotypes of the CD4⁺ T cells obtained by this method would be expected. Histologicexaminations of adjacent tissues were routinely performed in allcases to ensure the quality of the samplestaken.

Briefly, IEL were isolated from intestinal segments by using EDTA and mechanical agitation, and LPL were isolated from remainingintestinal pieces by using collagenase. Biopsy specimens weresimilarly treated with EDTA and collagenase, but cells derivedfrom these samples were pooled. Lymphocytes from all regions wereenriched by Percoll density gradient centrifugation (55). Intestinalcell viability was always greater than 90%, as determined by trypanblue dye exclusion. In all cases, cells were stained the day ofsampling and cell suspensions were kept on ice between each incubationso that no changes in cell surface expression could occur afterthe tissues were harvested. Previous studies have shown that theseprocedures do not affect the expression of cell surface markers,including those associated with cell activation (60). Lymphocyteswere also obtained from the spleen and axillary, inguinal, andmesenteric lymph nodes (from sacrificed animals only) by gentlycutting and pressing tissues through nylon mesh screens. Peripheralblood from all animals was stained by a whole blood lysis techniqueas describedbelow.

Cells were stained for four-color flow cytometric analysis using monoclonal antibodies to the panel of markers listed in Table1. Cells were stained by incubating 10⁶ cells from each of the above-described samples with excess amountsof monoclonal antibodies at 4°C for 30 min, followed by a wash(400 × g, 7 min) and fixation in 2% paraformaldehyde. Blood wasstained by incubating 100 µl of whole blood with monoclonal antibodiesfor 30 min at 4°C, followed by a 7-min lyse with FACS (fluorescence-activatedcell sorting) lysing solution (Becton Dickinson, San Jose, Calif.).Cells were then washed (400 × g, 7 min) and resuspended in 2%paraformaldehyde. All antibodies were directly conjugated to eitherfluorescein isothiocyanate (FITC), phycoerythrin (PE), peridininchlorophyll protein (PerCP), or allophycocyanin (APC) or (forCD3) were biotinylated and stained in a second step with streptavidin613 (Gibco). Monoclonal antibodies used were Leu-5b (CD2-PE),Leu-18 (CD45RA-FITC), Leu-8 (L-selectin or CD62L-PE), Leu-16 (CD20-FITC),Leu19 (CD56-PE), Leu-2b (CD8-FITC, CD8-PE), anti-HLA-DR-PE, Leu-28(CD28-PE), Leu3a (CD4-APC), and anti-interleukin-2 receptor (CD25-FITC),all obtained from Becton Dickinson. OKT4 (CD4-FITC) and OKT10(CD38-FITC) were obtained from Ortho Diagnostics (Raritan, N.J.),5A6.E9 (pan- $gamma$ $delta$ TCR-FITC) was obtained from Endogen (Woburn, Mass.),QBEND-10 (CD34-biotin) was obtained from Immunotech (Westbrook,Maine), 3B5 (CD8-APC) and BL-Ac/p26 (CD69-PE) were obtained fromCaltag Laboratories (San Francisco, Calif.), and 6G12 (CD3-biotin)was kindly provided by J. Wong, Massachusetts General Hospital(22). Controls consisted of appropriate unstained and irrelevantisotype-stained samples as well as single-color-stained samplesto verify the staining specificity of experimental antibodies.Data were acquired by using a Vantage or FacsCalibur flow cytometer(Becton Dickinson) and analyzed with Cell Quest software (BectonDickinson).

Statistical analyses. Differences in percentages and numbers of lymphocytes were compared between groups of animals at different time points, usinga Student pairwise t test and commercial statistical software(SigmaPlot; SPSS, Chicago, Ill.).

Immunohistochemistry and quantitative analysis. For determination of numbers of T cells per square millimeter of lamina propria, immunohistochemistry for CD3 was performedon 6-µm-thick sections of paraffin-embedded jejunum from 4 uninfectedand 10 acutely infected macaques as previously described (55).Diaminobenzidine was used as the chromagen, and slides were lightlycounterstained with hematoxylin. Thus, all CD3⁺ cells were dark brown and negative cells were light blue. Positive(brown) cells were then counted using an Olympus Vanox-S microscopeinterfaced to a Quantimet 570C image analysis system (Leica, Cambridge,Mass.). First, a detection threshold that would detect all browncells and discard blue cells for all sections was determined.Then, a two-dimensional, irregularly shaped field was carefullydrawn around the lamina propria (from the basal villi to the laminamuscularis [excluding crypts and solitary lymphoid follicles]),and the total area in square millimeters was determined. The positivecells within this field were then counted using a computer programdesigned by one of us to exclude artifacts and distinguish adjacentcells. The number of CD3⁺ T cells per square millimeter was then determined by dividingthe total positive cells in a particular field by the area insquare millimeters of the field in which they were counted. Atleast five fields (0.5 to 1.0 mm², total area) were counted for each section. The mean number ofT cells per square millimeter was determined by averaging allfields counted in eachsection.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Normal intestinal lamina propria CD4⁺ T cells have an activated memory phenotype. As previously described, the proportions of the major intestinal T-cell subsets of normal macaques are similar, if not identical,to those found in humans (55). Macaque IEL are predominantlyCD3⁺ CD8⁺, whereas LPL consist of approximately equal percentages of CD4⁺ and CD8⁺ T cells (55). In this study, three- and four-color flow cytometryof lymphocytes from uninfected adult macaques revealed that thevast majority (mean, 93%) of the CD3⁺ CD4⁺ double-positive (DP) T cells in the lamina propria of the jejunumand to a slightly lesser extent (mean, 78 to 79%) ileum and colonconsistently express high levels of CD69, an early and reliablemarker of lymphocyte activation (59) (Fig. 1; Table 2). Incontrast, CD69 expression was significantly lower (P < 0.01) onCD3⁺ CD4⁺ cells obtained from peripheral lymph nodes (mean, 27.2%) andrare (mean, 3.2%) on peripheral blood CD3⁺ CD4⁺ T cells of normal macaques (Fig. 1; Table 2). Interleukin-2receptor (CD25) expression was also consistently and significantly(P < 0.01) higher on intestinal lymphocytes than on peripherallymph nodes, spleen, or blood (Fig. 1; Table 2). As with CD69,CD25 expression was consistently highest on lamina propria CD4⁺ T cells from the jejunum (mean, 25%; range, 11 to 37%) comparedto peripheral blood (mean, 5.8%; range, 2 to 11%) or lymph nodes(mean, 8.4%; range, 4 to 13%) (Fig. 1; Table 2).

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FIG. 1. Comparison of lymphocyte activation (CD69, CD25, CD38, and HLA-DR expression) on CD4⁺ T cells from the intestinal lamina propria (left) to CD4⁺ T cells obtained from the axillary lymph node (LN; center) and blood (right) from an uninfected normal rhesus macaque. Note that essentially all intestinal CD4⁺ T cells are CD69⁺ HLA-DR⁺ CD38⁺. Plots were generated by gating first through lymphocytes and then through CD4⁺ cells.

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TABLE 2. Summary of results of three- and four-color immunophenotyping of CD4⁺ T cells in normal macaque tissues

HLA-DR expression was also consistently higher on intestinal lamina propria CD4⁺ T cells than on peripheral CD4⁺ T cells in individual animals (Fig. 1; Table 2). However, markedvariation in the expression of HLA-DR was noted between individualmacaques. Although some animals had very high HLA-DR expression(up to 95% of CD3⁺ CD4⁺ intestinal lymphocytes), others had very little HLA-DR expressionon CD4⁺ T cells. On average, 48% of lamina propria CD3⁺ CD4⁺ cells expressed HLA-DR, whereas 26% of axillary lymph node and19% of peripheral blood CD3⁺ CD4⁺ T cells were HLA-DR⁺ (Fig. 1; Table 2). However, the wide variation in HLA-DR expressionbetween individuals resulted in no statistically significant differencesbetweentissues.

Intestinal lamina propria CD4⁺ T cells from uninfected adult macaques were essentially all memory (CD45RA) cells (Fig. 2; Table 2). Over 95% of jejunum LPLs and 90% ofileum and colon LPLs were CD45RA negative, indicating a memoryphenotype. Duodenal CD4⁺ T lymphocytes obtained from uninfected juvenile macaques hadslightly higher CD45RA expression (mean, 15%) (Fig. 3). In contrast,68% (range, 43 to 86%) of the peripheral blood and 50% (range,36 to 75%) of peripheral lymph node CD3⁺ CD4⁺ lymphocytes coexpress CD45RA, indicating that they are naiveor resting lymphocytes (Table 2). Moreover, a large percentageof the CD3⁺ CD4⁺ CD45RA⁺ cells in peripheral tissues were L-selectin⁺, which is also consistent with naive cells. In contrast, lessthan 10% of the intestinal CD3⁺ CD4⁺ T cells (both LPL and IEL) expressed L-selectin (Table 2).

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FIG. 2. Flow cytometry dot plots of CD45RA and L-selectin expression on intestinal lamina propria CD3⁺ CD4⁺ T cells from an uninfected macaque (left), a macaque infected for 14 days (center), and an animal with AIDS (right). Note that the vast majority of intestinal memory (CD45RA) cells are eliminated in early SIV infection, resulting in an increased proportion of naive (CD45RA⁺) cells remaining. Plots were generated by gating first through lymphocytes and then through CD3⁺ CD4⁺ DP T cells (four-color flow cytometry).

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FIG. 3. Sequential changes in CD45RA expression on duodenal CD4⁺ T cells in juvenile macaques infected with SIV. Intestinal biopsies were taken from the same three macaques before infection (day 0) and in the first few weeks after SIVmac251 infection. Bars represent the proportion of the total remaining CD4⁺ T cells that express CD45RA. Note that most intestinal CD4⁺ T cells are memory (CD45RA) cells before infection, whereas increased proportions of naive (CD45RA⁺) CD4⁺ T cells are detected in the intestine of the same animals within weeks of SIV infection. Each bar represents the mean of the three animals examined ± standard deviation.

Acute SIV infection specifically results in the elimination of activated memory CD4⁺ T lymphocytes. As previously described, intestinal lamina propria CD4⁺ T cells were selectively and profoundly depleted within 14 days ofSIV infection (24, 48, 53). Gating on the remaining CD3⁺ CD4⁺ T cells in the lamina propria at all stages of SIV infectionrevealed a dramatic increase in the proportion of naive (CD45RA⁺) CD4⁺ T cells remaining in the intestinal lamina propria (Fig. 2 and3). Although CD45RA expression in the jejunum LPL was consistentlylow in uninfected animals, a marked increase in the proportionof the remaining CD3⁺ CD4⁺ T cells after 14 days of infection expressed CD45RA (Fig. 2 and3). This was particularly evident in animals followed prospectivelyby examining serial intestinal biopsies (Fig. 3). However, sinceintestinal CD4⁺ T cells are profoundly depleted after 14 days of infection, thelatter time points are usually based on a small number of cells(often fewer than 100 events per 20,000 collected). Therefore,it could not be determined whether this proportional increasein naive CD4⁺ T cells was due to recruitment (or expansion) of small numbersof naive T cells in the intestine, or if they simply representeda preexisting population which remained after the memory cellswere depleted. Moreover, CD4⁺ T cell loss was consistently (yet only slightly) more profoundin the jejunum than in the ileum or colon, which also correlateswith the findings of slightly higher percentages of memory CD4⁺ T cells in the jejunum. This finding further supports the hypothesisthat a selective depletion of activated memory CD4⁺ T cells was occurring in the intestinaltract.

A relative increase in CD45RA expression was also detected in peripheral lymph nodes and blood, despite the absence of significantchanges in overall CD4⁺ T-cell percentages or number. In fact, with gating through CD3⁺ CD4⁺ T cells, a remarkably consistent (11 of 11 animals examined)elimination of CD45RA Leu8 (memory) CD4⁺ T cells occurred in peripheral blood when the same animals werecompared at different time points in early infection (Fig. 4).However, since the starting percentages of memory CD4⁺ T cells in peripheral blood are substantially lower than thosein the LPL, no significant changes in absolute numbers of CD4⁺ T cells in the blood were observed during these early time points,as previously described (24, 48, 53). A similar increasein the proportion of naive cells was noted in the lymph nodesin early SIV infection, indicating that a loss of memory cellsoccurs in peripheral lymphoid tissues as well (Fig. 5).

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FIG. 4. Flow cytometry dot plots demonstrating a selective loss of memory CD4⁺ T cells in the peripheral blood of three macaques with early SIV infection. Each column shows the data from a single animal (animal numbers are listed above each column) examined before (top) and at 7, 14, and 30 days after SIV infection. Plots were generated by gating first through lymphocytes and then through CD4⁺ cells (three-color flow cytometry). Note that in each animal, a consistent loss of cells occurs in the upper left, lower left, and lower right quadrants by 14 days p.i., leaving only naive CD4⁺ (CD45RA⁺ CD62L⁺) T cells by 30 days p.i. (upper right quadrant). These results were representative of three separate experiments (n = 11).

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FIG. 5. Flow cytometry dot plots demonstrating a specific loss of memory CD4⁺ T cells in lymph nodes in early SIV infection. Plots on the left are from uninfected macaques, and those on the right are from different animals (cross-sectional study) infected with SIVmac239 for 21 or 50 days. Plots were generated by gating first through lymphocytes and then through CD3⁺ CD4⁺ cells (four-color flow cytometry). As in the blood, significantly fewer memory (CD45RA) cells are detected in lymph nodes from animals in early SIV infection than in those from uninfected animals. Note the decreased proportion of cells in the upper and lower left quadrants (memory cells) in the infected animals.

Regional variations exist in intestinal lymphocyte compartments. Since samples from the jejunum, ileum, and colon were processed and analyzed separately, distinct regional differences inlymphocyte subsets were detected between these regions. Importantly,lymphocytes from the ileum and colon consistently had slightly(<10% difference) higher percentages of both naive (CD45RA⁺) and resting (CD69 CD25) CD4⁺ T cells (Table 2). As previously mentioned, these findings areconsistent with the presence of organized lymphoid tissues (Peyer'spatches and organized lymphoid follicles) which are more frequentin the ileum and colon than in the jejunum. While these regionaldifferences were detectable, they were insignificant comparedto the marked differences between LPL from any region and peripherallymphocytes. As previously described, intestinal IEL were predominantlyCD3⁺ CD8⁺, yet some (up to 20%) were CD4⁺ (and usually CD4⁺ CD8⁺ DP), particularly in samples from the ileum and/or colon. Theintestinal epithelium that overlies human Peyer's patches (follicle-associatedepithelium) is known to contain more CD4⁺ T cells (5), and thus these regional differences in the IELare consistent with the presence of Peyer's patches in the ileumandcolon.

Increased numbers of CD8⁺ T cells appear in intestinal tissues following SIV infection. To examine the possibility that changes in T-cell subsets could be due to recruitment or expansion of other cell subsets,overall percentages of CD3⁺ T cells within the lymphocyte gate were compared. No significantdifferences in the percentages of CD3⁺ T cells were detected in any of the compartments examined (datanot shown). To quantitate T-cell numbers in the intestinal laminapropria, immunohistochemistry for CD3 was done on sections ofjejunum, and total T-cell numbers per square millimeter were thendetermined in the lamina propria of uninfected and acutely infectedanimals. Although there was a trend for an overall decrease, nosignificant changes in absolute numbers of CD3⁺ T cells per square millimeter were detected on immunohistochemicallystained intestinal sections after early SIV infection (Fig. 6).To estimate total numbers of CD4⁺ and CD8⁺ T cells per square millimeter of intestine, the number of totalT cells (as determined by immunohistochemistry and image analysis)was multiplied by the percentage of T cells that were either CD4⁺ or CD8⁺ (as determined by electronically gating through CD3⁺ T cells) for each corresponding jejunal segment. Using this method,we determined that a marked loss in absolute numbers of CD4⁺ T cells was occurring concurrently with an increase in numbersof CD8⁺ T cells in the intestinal lamina propria (Fig. 6).

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FIG. 6. Estimation of the changes in the total numbers of T cells per square millimeter in the intestinal lamina propria in early SIV infection. Each time point represents the mean of two (infected) or four (uninfected control) animals. Morphometric analysis of CD3⁺ T cells in immunohistochemically stained jejunum sections was used to determine the numbers of CD3⁺ T cells per square millimeter of lamina propria (see text), and CD4⁺ and CD8⁺ T cells per square millimeter were determined by multiplying the number of CD3⁺ cells per square millimeter by the percentage of gated CD3⁺ lymphocytes coexpressing CD4 or CD8 in corresponding jejunum lamina propria as determined by flow cytometry (DP cells would be included in both bars). Note that a profound loss in CD4⁺ T cells per square millimeter occurs by 21 days after SIV infection, corresponding with an increase in absolute numbers of CD8⁺ T cells. Overall, this results in minimal changes in absolute numbers of CD3⁺ T cells in the lamina propria.

Other findings. Although $gamma$ $delta$ T cells represented 5 to 25% of all IEL in the macaques examined, no significant changes in percentages or numbersof $gamma$ $delta$ T cells were detected in response to SIV infection. Moreover,no significant change in CD20 expression (resting B cells) wasdetected in early SIV infection compared to controls. A considerable(yet variable) proportion of macaque intestinal T cells expressboth CD4 and CD8 (i.e., are DP cells). Since the only other organthat harbors large numbers of these unique T cells is the thymus,our staining panel was designed to further characterize thesecells. However, by three- and four-color analysis, DP cells weredetermined to share most of the phenotypic traits of the single-positiveCD4⁺ T cells in the intestine: they have an activated (CD69⁺) memory (CD45RA L-selectin) phenotype and are also rapidly eliminated in early SIV infection.In fact, both the speed and the degree of intestinal DP cell depletionwas greater than those of CD4⁺ single-positive T cells (data not shown). Moreover, these cellslacked CD34 expression (unlike thymocytes) and expressed CD69similarly to single-positive CD4⁺ T cells (data not shown). This finding indicates that intestinalDP cells are very different from thymus DP cells and are probablyhighly activated effector cells rather than immature precursorcells.

Approximately 80% of intestinal lamina propria CD4⁺ T cells expressed CD38, but these percentages were not significantly differentfrom those of CD4⁺ T cells from the lymph nodes, spleen, and blood (Table 2). Inaddition, the vast majority of CD3⁺ CD4⁺ T cells in the intestinal lamina propria coexpress CD28, whichwas similar to percentages of CD28 expression by peripheral lymphnode and blood CD4⁺ T cells (Table 2). Interestingly, CD28 expression was loweron jejunum LPL than LPL from the ileum, colon, or peripheral tissues(Table 2).

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

Combined, these data clearly show that the vast majority of activated (CD69⁺ HLA-DR⁺ CD38⁺) memory (CD45RA Leu8) CD3⁺ CD4⁺ T lymphocytes in normal primates reside within the intestinalmucosa and that it is this specific T-cell subset that is preferentiallyeliminated in primary SIV infection. Moreover, the intestinalCD4 depletion is preceded by infection of large numbers of intestinallymphocytes in early SIV infection (20, 53). Combined, thesedata indicate that the primary target cell for SIV replicationis a T cell positive for CD2, CD3, CD4, CD69, and CD38 and variablybut consistently higher than other CD4⁺ T cells in its expression of HLA-DR and CD25. In addition, thesecells may have slightly lower expression of CD28. Decreased expressionof CD28 has also been described as a feature of activated CD4⁺ T cells (51). Combined, the pattern of cell surface moleculeexpression on intestinal CD4⁺ T cells is consistent with a high degree of, and/or recent, cellularactivation. Moreover, these cells are consistently negative forboth CD45RA and L-selectin, which indicates that they have beenantigen primed (i.e., are memory cells). Thus, the target cellfor primary SIV infection may be defined as an activated memoryCD4⁺ T cell. Furthermore, we have shown that loss of this specificsubset of CD4⁺ T cells can consistently be detected in the blood and peripherallymph nodes as well as in the intestinal mucosa in the first fewweeks of SIVinfection.

Activated mucosal memory T cells are by definition actively engaged in protecting mucosal surfaces from invasion by pathogens,as well as in regulating local immune responses to the large quantitiesof dietary antigens that are consumed. These cells are abundantthroughout the intestinal tract, which is the largest immunologicorgan of the body (30, 35). The size of the gastrointestinaltract combined with the high density of activated memory CD4⁺ T cells in the intestinal lamina propria may make this the mostplentiful T-cell subset in the body of uninfected healthy individuals.By combining flow cytometry with quantitative assessments of T-cellnumbers in the intestine, we have confirmed that SIV infectionresults in massive CD4⁺ T-cell loss per unit area of intestinal lamina propria. Thisrepresents an extensive loss of total CD4⁺ T cells in primary SIV infection since the gut is such a largereservoir of CD4⁺ T cells. Moreover, as demonstrated in this report, the intestineis the main reservoir for activated memory CD4⁺ Tcells.

Combined, these data strongly suggest that there is a preference for SIV replication and amplification within a specific subsetof CD4⁺ T cells. If primary infection and optimal viral replication dependon the presence of activated memory CD4⁺ T cells (which are found primarily in the intestine and are rapidlyeliminated), this could contribute to the decline in viral loadsobserved following primary infection, as well as the establishmentof a viral set point that signals the onset of clinical latency.A similar in vivo model for HIV infection whereby the reductionin viral loads in acute infection is hypothesized to be independentof an HIV-specific immune response has been proposed (39). Ifthis model is correct, then possibly HIV replication in clinicallatency is limited by the rate of T-cell production and conversionfrom naive to memory cells, which would be very slow in healthyindividuals unless there was a specific stimulus for CD4⁺ T cell proliferation. Establishment of an opportunistic mucosalinfection would provide this stimulus. Indeed, opportunistic infectionsas well as immune challenge and vaccination have been associatedwith increased viral loads in HIV infection (18, 37, 50).Alternatively, the virus itself may be involved in convertingresting CD4⁺ T cells to appropriately activated memory T cells that promoteviral replication. The nef genes of both HIV and SIV have beendemonstrated to play a role in T-cell activation and viral replicationin vitro (1, 13, 14, 23, 29, 57) and, for SIV, invivo (14, 44). The biochemical pathways by which nef induceslymphocyte activation have not been completely elucidated, butstudies have shown that nef interacts with a series of cellularpartners including CD4, components of the adapter complexes AP-1and AP-2, and several protein kinases (41).

Viral dynamics are also clearly influenced by the presence of virus specific CD8⁺ T cells, as shown by recent CD8⁺ T-cell depletion studies (21, 45). It is likely that boththe depletion of optimal target cells and the development of SIV-specificimmune responses contribute to the decline in viral loads andthe establishment of viral set points in early SIV or HIV infection.In the future, it will be important to examine viral load, anti-SIV-specificCD8⁺ T-cell responses, and CD4⁺ T cells in the intestinal mucosa to address this issue. It ispossible that intestinal CD4⁺ T-cell depletion is a result of direct viral lysis as well asCTL-mediated cell destruction. Thus, the depletion of CD8 cellsmay decrease the rate at which infected CD4⁺ T cells are lost, which could account for the increased viralloads.

In conclusion, we have defined the major target cell of primary SIV infection as an activated memory CD4⁺ T cell. The normal intestinal tract contains large numbers ofthis cell type, making this the preferred site of SIV and HIVreplication, at least in primary infection. These data stronglysuggest that inducing an appropriate anti-HIV immune responsespecifically within mucosal sites may be of paramount importancein producing an effective HIVvaccine.

	ACKNOWLEDGMENTS

We thank Michael O'Connell for coordinating these studies and the animal care staff at the New England Regional Primate ResearchCenter for their excellent care of themacaques.

This work was supported by NIH grants DK50550, RR00168, HD36310, and HL59787. A. A. Lackner is the recipient of an ElizabethGlaser ScientistAward.

	FOOTNOTES

^* Corresponding author. Mailing address: Division of Comparative Pathology, One Pine Hill Drive, P.O. Box 9102, Southborough,MA 01772. Phone: (508) 624-8013. Fax: (508) 624-8181. E-mail:ronald_veazey{at}hms.harvard.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Aiken, C., and D. Trono. 1995. Nef stimulates human immunodeficiency virus type 1 proviral DNA synthesis. J. Virol. 69:5048-5056[Abstract].

2. Akari, H., K. Mori, I. Otani, K. Terao, F. Ono, A. Adachi, and Y. Yoshikawa. 1998. Induction of MHC-IIDR expression on circulating CD8+ lymphocytes in macaques infected with SIVmac239 nef-open but not with its nef-deletion mutant. AIDS Res. Hum. Retroviruses 14:619-625[Medline].

3. Bell, E. B., S. M. Sparshott, and C. Bunce. 1998. CD4+ T-cell memory, CD45R subsets, and the persistence of antigen $---$ a unifying concept. Immunol. Today 19:60-64[CrossRef][Medline].

4. Berg, M., Y. Murakawa, D. Camerini, and S. P. James. 1991. Lamina propria lymphocytes are derived from circulating cells that lack the Leu-8 lymph node homing receptor. Gastroenterology 101:90-99[Medline].

5. Bjerke, K., P. Brandtzaeg, and O. Fausa. 1988. T cell distribution is different in follicle-associated epithelium of human Peyer's patches and villus epithelium. Clin. Exp. Immunol. 74:270-275[Medline].

6. Blair, P. J., J. L. Riley, R. G. Carroll, D. C. St. Louis, B. L. Levine, B. Saha, K. P. Lee, P. J. Perrin, D. M. Harlan, and C. H. June. 1997. CD28 co-receptor signal transduction in T-cell activation. Biochem. Soc. Trans. 25:651-657[Medline].

7. Bleul, C. C., L. Wu, J. A. Hoxie, T. A. Springer, and C. R. Mackay. 1997. The HIV coreceptors CXCR4 and CCR5 are differentially expressed and regulated on human T lymphocytes. Proc. Natl. Acad. Sci. USA 94:1925-1930[Abstract/Free Full Text].

8. Borvak, J., C.-S. Chou, K. Bell, G. Van Dyke, H. Zola, O. Ramilo, and E. S. Vitetta. 1995. Expression of CD25 defines peripheral blood mononuclear cells with productive versus latent HIV infection. J. Immunol. 155:3196-3204[Abstract].

9. Butcher, E. C., and L. J. Picker. 1996. Lymphocyte homing and homeostasis. Science 272:60-66[Abstract].

10. Chou, C.-S., O. Ramilo, and E. S. Vitetta. 1997. Highly purified CD25 $-$ resting T cells cannot be infected de novo with HIV-1. Proc. Natl. Acad. Sci. USA 94:1361-1365[Abstract/Free Full Text].

11. Chun, T.-W., D. Engel, S. B. Mizell, L. A. Ehler, and A. S. Fauci. 1998. Induction of HIV-1 replication in latently infected CD4+ T cells using a combination of cytokines. J. Exp. Med. 188:83-91[Abstract/Free Full Text].

12. Clayton, F., G. Snow, S. Reka, and D. P. Kotler. 1997. Selective depletion of rectal lamina propria rather than lymphoid aggregate CD4 lymphocytes in HIV infection. Clin. Exp. Immunol. 107:288-292[CrossRef][Medline].

13. Du, Z., P. O. Ilyinskii, V. G. Sasseville, M. Newstein, M. D. Daniel, A. A. Lackner, and R. C. Desrosiers. 1996. Requirements for lymphocyte activation by unusual strains of simian immunodeficiency virus. J. Virol. 70:4157-4161[Abstract].

14. Du, Z., S. M. Lang, V. G. Sasseville, A. A. Lackner, P. O. Ilyinskii, M. D. Daniel, J. U. Jung, and R. C. Desrosiers. 1995. Identification of a nef allele that causes lymphocyte activation and acute disease in macaque monkeys. Cell 82:665-674[CrossRef][Medline].

15. Edmead, C. E., J. R. Lamb, and G. F. Hoyne. 1997. The T cell surface protein, CD28. Int. J. Biochem. Cell Biol. 29:1053-1057[CrossRef][Medline].

16. Finzi, D., M. Hermankova, T. Pierson, L. M. Carruth, C. Buck, R. E. Chaisson, T. C. Quinn, K. Chadwick, J. Margolick, R. Brookmeyer, J. Gallant, M. Markowitz, D. D. Ho, D. D. Richman, and R. F. Siliciano. 1997. Identification of a reservoir for HIV-1 in patients on highly active antiretroviral therapy. Science 278:1295-1300[Abstract/Free Full Text].

17. Finzi, D., and R. F. Siliciano. 1998. Viral dynamics in HIV-1 infection. Cell 93:665-671[CrossRef][Medline].

18. Grossman, Z., M. B. Feinberg, and W. E. Paul. 1998. Multiple modes of cellular activation and virus transmission in HIV infection: a role for chronically and latently infected cells in sustaining viral replication. Proc. Natl. Acad. Sci. USA 95:6314-6319[Abstract/Free Full Text].

19. Haseltine, W. A., and F. Wong-Staal. 1988. The molecular biology of the AIDS virus. Sci. Am. 259:52-62[Medline].

20. Heise, C., P. Vogel, C. J. Miller, A. Lackner, and S. Dandekar. 1993. Distribution of SIV infection in the gastrointestinal tract of rhesus macaques at early and terminal stages of AIDS. J. Med. Primatol. 22:187-193[Medline].

21. Jin, X., D. E. Bauer, S. E. Tuttleton, S. Lewin, A. Gettie, J. Blanchard, C. E. Irwin, J. T. Safrit, J. Mittler, L. Weinberger, L. G. Kostrikis, L. Zhang, A. S. Perelson, and D. D. Ho. 1999. Dramatic rise in plasma viremia after CD8(+) T cell depletion in simian immunodeficiency virus-infected macaques. J. Exp. Med. 189:991-998[Abstract/Free Full Text].

22. Kawai, T., J. Wong, J. MacLean, A. B. Cosimi, and S. Wee. 1994. Characterization of a monoclonal antibody (6G12) recognizing the cynomolgus monkey CD3 antigen. Transplant. Proc. 26:1845[Medline].

23. Kestler, H. W., D. J. Ringler, K. Mori, D. L. Panicali, P. K. Sehgal, M. D. Daniel, and R. C. Desrosiers. 1991. Importance of the nef gene for maintenance of high viral loads and for the development of AIDS. Cell 65:651-662[CrossRef][Medline].

24. Kewenig, S., T. Schneider, K. Hohloch, K. Lampe-Dreyer, R. Ullrich, N. Stolte, C. Stahl-Hennig, F. J. Kaup, A. Stallmach, and M. Zeitz. 1999. Rapid mucosal CD4+ T-cell depletion and enteropathy in simian immunodeficiency virus-infected rhesus macaques. Gastroenterology 116:1115-1123[CrossRef][Medline].

25. Lefrere, J. J., F. Roudot-Thoraval, M. Mariotti, M. Thauvin, J. Lerable, J. Salpetrier, and L. Morand-Joubert. 1998. The risk of disease progression is determined during the first year of human immunodeficiency virus type 1 infection. J. Infect. Dis. 177:1541-1548[Medline].

26. Lenschow, D. J., T. L. Walunas, and J. A. Bluestone. 1996. CD28/B7 system of T cell costimulation. Annu. Rev. Immunol. 14:233-258[CrossRef][Medline].

27. Lim, S. G., A. Condez, C. A. Lee, M. A. Johnson, C. Elia, and L. W. Poulter. 1993. Loss of mucosal CD4 lymphocytes is an early feature of HIV infection. Clin. Exp. Immunol. 92:448-454[Medline].

28. Lloyd, T. E., L. Yang, D. N. Tang, T. Bennett, W. Schober, and D. E. Lewis. 1997. Regulation of CD28 costimulation in human CD8+ T cells. J. Immunol. 158:1551-1558[Abstract].

29. Luo, T., J. R. Downing, and J. V. Garcia. 1997. Induction of phosphorylation of human immunodeficiency virus type 1 nef and enhancement of CD4 downregulation by phorbol myristate acetate. J. Virol. 71:2535-2539[Abstract].

30. MacDonald, T. T., and J. Spencer. 1994. Lymphoid cells and tissues of the gastrointestinal tract, p. 394-421. In R. H. Heatley (ed.), Gastrointestinal and hepatic immunology. Cambridge University Press, Cambridge, England

31. Mahalingham, M., M. Peakman, E. T. Davies, A. Pozniak, T. J. McManus, and D. Vergani. 1993. T cell activation and disease severity in HIV infection. Clin. Exp. Immunol. 93:337-343[Medline].

32. Malavasi, F., A. Funaro, S. Roggero, A. L. Horenstein, L. Calosso, and K. Mehta. 1994. Human CD38: one molecule in search of a function. Immunol. Today 15:95-97[CrossRef][Medline].

33. McDougal, J. S., A. Mawle, S. P. Cort, J. K. A. Nicholson, G. D. Cross, J. A. Schleppler-Campbell, D. Hicks, and J. Sligh. 1985. Cellular tropism of the human retrovirus HTLV-III/LAV. I. Role of T cell activation and expression of the T4 antigen. J. Immunol. 135:3151-3162[Abstract].

34. Mellors, J. W., C. R. Rinaldo, 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].

35. Mowat, A. M., and J. L. Viney. 1997. The anatomical basis of intestinal immunity. Immunol. Rev. 156:145-166[CrossRef][Medline].

36. Nabel, G., and D. Baltimore. 1987. An inducible transcription factor activates expression of human immunodeficiency virus in T cells. Nature 326:711-713[CrossRef][Medline].

37. Orenstein, J. M., C. Fox, and S. M. Wahl. 1997. Macrophages as a source of HIV during opportunistic infections. Science 276:1857-1861[Abstract/Free Full Text].

38. Pantaleo, G., C. Graziosi, and A. S. Fauci. 1997. Virologic and immunologic events in primary HIV infection. Springer Semin. Immunopathol. 18:257-266[CrossRef][Medline].

39. Phillips, A. N. 1996. Reduction of HIV concentration during acute infection: independence from a specific immune response. Science 271:497-498[Abstract].

40. Picker, L. J., J. R. Treer, B. Ferguson-Darnell, P. A. Collins, D. Buck, and L. W. M. M. Terstappen. 1993. Control of lymphocyte recirculation in man. 1. Differential regulation of the peripheral lymph node homing receptor L-selectin on T cells during the virgin to memory cell transition. J. Immunol. 150:1105-1121[Abstract].

41. Piguet, V., and D. Trono. 1999. The nef protein of primate lentiviruses. Rev. Med. Virol. 9:111-120[CrossRef][Medline].

42. Reinis, M., M. Morra, A. Funaro, R. Di Primio, and F. Malavasi. 1997. Functional associations of CD38 with CD3 on the T cell membrane. J. Biol. Regul. Homeost. Agents 11:137-142[Medline].

43. Roederer, M., J. G. Dubs, M. T. Anderson, P. A. Raju, and L. A. Herzenberg. 1995. CD8 naive T cell counts decrease progressively in HIV-infected patients. J. Clin. Investig. 95:2061-2066.

44. Sasseville, V. G., Z. Du, L. V. Chalifoux, D. R. Pauley, H. Y. Young, P. K. Sehgal, R. C. Desrosiers, and A. A. Lackner. 1996. Induction of lymphocyte proliferation and severe gastrointestinal disease in macaques by a nef gene variant of SIVmac239. Am. J. Pathol. 149:163-175[Abstract].

45. Schmitz, J. E., M. J. Kuroda, S. Santra, V. G. Sasseville, M. A. Simon, M. A. Lifton, P. Racz, K. Tenner-Racz, M. Dalesandro, B. J. Scallon, J. Ghrayeb, M. A. Forman, D. C. Montefiori, E. P. Rieber, N. L. Letvin, and K. A. Reimann. 1999. Control of viremia in simian immunodeficiency virus infection by CD8+ lymphocytes. Science 283:857-860[Abstract/Free Full Text].

46. Schneider, T., H.-U. Jahn, W. Schmidt, E.-O. Reicken, M. Zeitz, and R. Ulrich. 1995. Loss of CD4 T lymphocytes in patients infected with human immunodeficiency virus type 1 is more pronounced in the duodenal mucosa than in the peripheral blood. Gut 37:524-529[Abstract/Free Full Text].

47. Schnittman, S. M., H. C. Lane, J. Greenhouse, J. S. Justement, M. Baseler, and A. S. Fauci. 1990. Preferential infection of CD4+ memory cells by human immunodeficiency virus type 1: evidence for a role in the selective T-cell functional defects observed in infected individuals. Proc. Natl. Acad. Sci. USA 87:6058-6062[Abstract/Free Full Text].

48. Smit-McBride, Z., J. J. Mattapallil, M. McChesney, D. Ferrick, and S. Dandekar. 1998. Gastrointestinal T lymphocytes retain high potential for cytokine responses but have severe CD4⁺ T-cell depletion at all stages of simian immunodeficiency virus infection compared to peripheral lymphocytes. J. Virol. 72:6646-6656[Abstract/Free Full Text].

49. 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].

50. Staprans, S. I., B. L. Hamilton, S. E. Follansbee, T. Elbeik, P. Barbosa, R. M. Grant, and M. B. Feinberg. 1995. Activation of virus replication after vaccination of HIV-1 infected individuals. J. Exp. Med. 182:1727-1737[Abstract/Free Full Text].

51. van den Hove, L. E., P. Vandenberghe, S. W. Van Gool, J. L. Ceuppens, H. Demuynck, G. E. Verhoef, and M. A. Boogaerts. 1998. Peripheral blood lymphocyte subset shifts in patients with untreated hematological tumors: evidence for systemic activation of the T cell compartment. Leuk. Res. 22:175-184[CrossRef][Medline].

52. van Noesel, C. J., R. A. Gruters, F. G. Terpstra, P. T. Schellekens, R. A. van Lier, and F. Miedema. 1990. Functional and phenotypic evidence for a selective loss of memory T cells in asymptomatic human immunodeficiency virus-infected men. J. Clin. Investig. 86:293-299.

53. Veazey, R. S., M. DeMaria, L. V. Chalifoux, D. E. Shvetz, D. R. Pauley, H. L. Knight, M. Rosenzweig, R. P. Johnson, R. C. Desrosiers, and A. A. Lackner. 1998. Gastrointestinal tract as a major site of CD4+ T cell depletion and viral replication in SIV infection. Science 280:427-431[Abstract/Free Full Text].

54. Veazey, R. S., and A. A. Lackner. 1998. The gastrointestinal tract and the pathogenesis of AIDS. AIDS 12:S35-S42.

55. Veazey, R. S., M. Rosenzweig, D. E. Shvetz, D. R. Pauley, M. DeMaria, L. V. Chalifoux, R. P. Johnson, and A. A. Lackner. 1997. Characterization of gut-associated lymphoid tissues (GALT) of normal rhesus macaques. Clin. Immunol. Immunopathol. 82:230-242[CrossRef][Medline].

56. Westmoreland, S. V., E. Halpern, and A. A. Lackner. 1998. Simian immunodeficiency virus encephalitis in rhesus macaques is associated with rapid disease progression. J. Neurovirol. 4:260-268[Medline].

57. Whetter, L., F. J. Novembre, M. Saucier, S. Gummurulu, and S. Dewhurst. 1998. Costimulatory pathways in lymphocyte proliferation induced by the simian immunodeficiency virus SIVsmmPBj14. J. Virol. 72:6155-6158[Abstract/Free Full Text].

58. Willerford, D. M., M. J. Gale, Jr., R. E. Benveniste, E. A. Clark, and W. M. Gallatin. 1990. Simian immunodeficiency virus is restricted to a subset of blood CD4+ T lymphocytes that includes memory cells. J. Immunol. 144:3779-3783[Abstract].

59. Zeigler, S. F., F. Ramsdell, and M. R. Alderson. 1994. The activation antigen CD69. Stem Cells 12:456-465[Abstract].

60. Zeitz, M., W. C. Greene, N. J. Peffer, and S. P. James. 1988. Lymphocytes isolated from the intestinal lamina propria of normal nonhuman primates have increased expression of genes associated with T cell activation. Gastroenterology 94:647-655[Medline].

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George, M. D., Reay, E., Sankaran, S., Dandekar, S. (2005). Early Antiretroviral Therapy for Simian Immunodeficiency Virus Infection Leads to Mucosal CD4+ T-Cell Restoration and Enhanced Gene Expression Regulating Mucosal Repair and Regeneration. J. Virol. 79: 2709-2719 [Abstract] [Full Text]
Koopman, G., Mortier, D., Hofman, S., Niphuis, H., Fagrouch, Z., Norley, S., Sutter, G., Liljestrom, P., Heeney, J. L. (2004). Vaccine protection from CD4+ T-cell loss caused by simian immunodeficiency virus (SIV) mac251 is afforded by sequential immunization with three unrelated vaccine vectors encoding multiple SIV antigens. J. Gen. Virol. 85: 2915-2924 [Abstract] [Full Text]
Mehandru, S., Poles, M. A., Tenner-Racz, K., Horowitz, A., Hurley, A., Hogan, C., Boden, D., Racz, P., Markowitz, M. (2004). Primary HIV-1 Infection Is Associated with Preferential Depletion of CD4+ T Lymphocytes from Effector Sites in the Gastrointestinal Tract. J. Exp. Med. 200: 761-770 [Abstract] [Full Text]
Veazey, R. S., Lackner, A. A. (2004). Getting to the Guts of HIV Pathogenesis. J. Exp. Med. 200: 697-700 [Abstract] [Full Text]
Stevens, R., Howard, K. E., Nordone, S., Burkhard, M., Dean, G. A. (2004). Oral Immunization with Recombinant Listeria monocytogenes Controls Virus Load after Vaginal Challenge with Feline Immunodeficiency Virus. J. Virol. 78: 8210-8218 [Abstract] [Full Text]
Hirsch, V. M., Santra, S., Goldstein, S., Plishka, R., Buckler-White, A., Seth, A., Ourmanov, I., Brown, C. R., Engle, R., Montefiori, D., Glowczwskie, J., Kunstman, K., Wolinsky, S., Letvin, N. L. (2004). Immune Failure in the Absence of Profound CD4+ T-Lymphocyte Depletion in Simian Immunodeficiency Virus-Infected Rapid Progressor Macaques. J. Virol. 78: 275-284 [Abstract] [Full Text]
Igarashi, T., Endo, Y., Nishimura, Y., Buckler, C., Sadjadpour, R., Donau, O. K., Dumaurier, M.-J., Plishka, R. J., Buckler-White, A., Martin, M. A. (2003). Early Control of Highly Pathogenic Simian Immunodeficiency Virus/Human Immunodeficiency Virus Chimeric Virus Infections in Rhesus Monkeys Usually Results in Long-Lasting Asymptomatic Clinical Outcomes. J. Virol. 77: 10829-10840 [Abstract] [Full Text]
Veazey, R. S., Lifson, J. D., Pandrea, I., Purcell, J., Piatak, M. Jr., Lackner, A. A. (2003). Simian Immunodeficiency Virus Infection in Neonatal Macaques. J. Virol. 77: 8783-8792 [Abstract] [Full Text]
Shacklett, B. L., Cox, C. A., Sandberg, J. K., Stollman, N. H., Jacobson, M. A., Nixon, D. F. (2003). Trafficking of Human Immunodeficiency Virus Type 1-Specific CD8+ T Cells to Gut-Associated Lymphoid Tissue during Chronic Infection. J. Virol. 77: 5621-5631 [Abstract] [Full Text]
Price, D. A., Scullard, G., Oxenius, A., Braganza, R., Beddows, S. A., Kazmi, S., Clarke, J. R., Johnson, G. E., Weber, J. N., Phillips, R. E. (2003). Discordant Outcomes following Failure of Antiretroviral Therapy Are Associated with Substantial Differences in Human Immunodeficiency Virus-Specific Cellular Immunity. J. Virol. 77: 6041-6049 [Abstract] [Full Text]
Sugimoto, C., Tadakuma, K., Otani, I., Moritoyo, T., Akari, H., Ono, F., Yoshikawa, Y., Sata, T., Izumo, S., Mori, K. (2003). nef Gene Is Required f

1.	Aiken, C., and D. Trono. 1995. Nef stimulates human immunodeficiency virus type 1 proviral DNA synthesis. J. Virol. 69:5048-5056[Abstract].
2.	Akari, H., K. Mori, I. Otani, K. Terao, F. Ono, A. Adachi, and Y. Yoshikawa. 1998. Induction of MHC-IIDR expression on circulating CD8+ lymphocytes in macaques infected with SIVmac239 nef-open but not with its nef-deletion mutant. AIDS Res. Hum. Retroviruses 14:619-625[Medline].
3.	Bell, E. B., S. M. Sparshott, and C. Bunce. 1998. CD4+ T-cell memory, CD45R subsets, and the persistence of antigen $---$ a unifying concept. Immunol. Today 19:60-64[CrossRef][Medline].
4.	Berg, M., Y. Murakawa, D. Camerini, and S. P. James. 1991. Lamina propria lymphocytes are derived from circulating cells that lack the Leu-8 lymph node homing receptor. Gastroenterology 101:90-99[Medline].
5.	Bjerke, K., P. Brandtzaeg, and O. Fausa. 1988. T cell distribution is different in follicle-associated epithelium of human Peyer's patches and villus epithelium. Clin. Exp. Immunol. 74:270-275[Medline].
6.	Blair, P. J., J. L. Riley, R. G. Carroll, D. C. St. Louis, B. L. Levine, B. Saha, K. P. Lee, P. J. Perrin, D. M. Harlan, and C. H. June. 1997. CD28 co-receptor signal transduction in T-cell activation. Biochem. Soc. Trans. 25:651-657[Medline].
7.	Bleul, C. C., L. Wu, J. A. Hoxie, T. A. Springer, and C. R. Mackay. 1997. The HIV coreceptors CXCR4 and CCR5 are differentially expressed and regulated on human T lymphocytes. Proc. Natl. Acad. Sci. USA 94:1925-1930[Abstract/Free Full Text].
8.	Borvak, J., C.-S. Chou, K. Bell, G. Van Dyke, H. Zola, O. Ramilo, and E. S. Vitetta. 1995. Expression of CD25 defines peripheral blood mononuclear cells with productive versus latent HIV infection. J. Immunol. 155:3196-3204[Abstract].
9.	Butcher, E. C., and L. J. Picker. 1996. Lymphocyte homing and homeostasis. Science 272:60-66[Abstract].
10.	Chou, C.-S., O. Ramilo, and E. S. Vitetta. 1997. Highly purified CD25 $-$ resting T cells cannot be infected de novo with HIV-1. Proc. Natl. Acad. Sci. USA 94:1361-1365[Abstract/Free Full Text].
11.	Chun, T.-W., D. Engel, S. B. Mizell, L. A. Ehler, and A. S. Fauci. 1998. Induction of HIV-1 replication in latently infected CD4+ T cells using a combination of cytokines. J. Exp. Med. 188:83-91[Abstract/Free Full Text].
12.	Clayton, F., G. Snow, S. Reka, and D. P. Kotler. 1997. Selective depletion of rectal lamina propria rather than lymphoid aggregate CD4 lymphocytes in HIV infection. Clin. Exp. Immunol. 107:288-292[CrossRef][Medline].
13.	Du, Z., P. O. Ilyinskii, V. G. Sasseville, M. Newstein, M. D. Daniel, A. A. Lackner, and R. C. Desrosiers. 1996. Requirements for lymphocyte activation by unusual strains of simian immunodeficiency virus. J. Virol. 70:4157-4161[Abstract].
14.	Du, Z., S. M. Lang, V. G. Sasseville, A. A. Lackner, P. O. Ilyinskii, M. D. Daniel, J. U. Jung, and R. C. Desrosiers. 1995. Identification of a nef allele that causes lymphocyte activation and acute disease in macaque monkeys. Cell 82:665-674[CrossRef][Medline].
15.	Edmead, C. E., J. R. Lamb, and G. F. Hoyne. 1997. The T cell surface protein, CD28. Int. J. Biochem. Cell Biol. 29:1053-1057[CrossRef][Medline].
16.	Finzi, D., M. Hermankova, T. Pierson, L. M. Carruth, C. Buck, R. E. Chaisson, T. C. Quinn, K. Chadwick, J. Margolick, R. Brookmeyer, J. Gallant, M. Markowitz, D. D. Ho, D. D. Richman, and R. F. Siliciano. 1997. Identification of a reservoir for HIV-1 in patients on highly active antiretroviral therapy. Science 278:1295-1300[Abstract/Free Full Text].
17.	Finzi, D., and R. F. Siliciano. 1998. Viral dynamics in HIV-1 infection. Cell 93:665-671[CrossRef][Medline].
18.	Grossman, Z., M. B. Feinberg, and W. E. Paul. 1998. Multiple modes of cellular activation and virus transmission in HIV infection: a role for chronically and latently infected cells in sustaining viral replication. Proc. Natl. Acad. Sci. USA 95:6314-6319[Abstract/Free Full Text].
19.	Haseltine, W. A., and F. Wong-Staal. 1988. The molecular biology of the AIDS virus. Sci. Am. 259:52-62[Medline].
20.	Heise, C., P. Vogel, C. J. Miller, A. Lackner, and S. Dandekar. 1993. Distribution of SIV infection in the gastrointestinal tract of rhesus macaques at early and terminal stages of AIDS. J. Med. Primatol. 22:187-193[Medline].
21.	Jin, X., D. E. Bauer, S. E. Tuttleton, S. Lewin, A. Gettie, J. Blanchard, C. E. Irwin, J. T. Safrit, J. Mittler, L. Weinberger, L. G. Kostrikis, L. Zhang, A. S. Perelson, and D. D. Ho. 1999. Dramatic rise in plasma viremia after CD8(+) T cell depletion in simian immunodeficiency virus-infected macaques. J. Exp. Med. 189:991-998[Abstract/Free Full Text].
22.	Kawai, T., J. Wong, J. MacLean, A. B. Cosimi, and S. Wee. 1994. Characterization of a monoclonal antibody (6G12) recognizing the cynomolgus monkey CD3 antigen. Transplant. Proc. 26:1845[Medline].
23.	Kestler, H. W., D. J. Ringler, K. Mori, D. L. Panicali, P. K. Sehgal, M. D. Daniel, and R. C. Desrosiers. 1991. Importance of the nef gene for maintenance of high viral loads and for the development of AIDS. Cell 65:651-662[CrossRef][Medline].
24.	Kewenig, S., T. Schneider, K. Hohloch, K. Lampe-Dreyer, R. Ullrich, N. Stolte, C. Stahl-Hennig, F. J. Kaup, A. Stallmach, and M. Zeitz. 1999. Rapid mucosal CD4+ T-cell depletion and enteropathy in simian immunodeficiency virus-infected rhesus macaques. Gastroenterology 116:1115-1123[CrossRef][Medline].
25.	Lefrere, J. J., F. Roudot-Thoraval, M. Mariotti, M. Thauvin, J. Lerable, J. Salpetrier, and L. Morand-Joubert. 1998. The risk of disease progression is determined during the first year of human immunodeficiency virus type 1 infection. J. Infect. Dis. 177:1541-1548[Medline].
26.	Lenschow, D. J., T. L. Walunas, and J. A. Bluestone. 1996. CD28/B7 system of T cell costimulation. Annu. Rev. Immunol. 14:233-258[CrossRef][Medline].
27.	Lim, S. G., A. Condez, C. A. Lee, M. A. Johnson, C. Elia, and L. W. Poulter. 1993. Loss of mucosal CD4 lymphocytes is an early feature of HIV infection. Clin. Exp. Immunol. 92:448-454[Medline].
28.	Lloyd, T. E., L. Yang, D. N. Tang, T. Bennett, W. Schober, and D. E. Lewis. 1997. Regulation of CD28 costimulation in human CD8+ T cells. J. Immunol. 158:1551-1558[Abstract].
29.	Luo, T., J. R. Downing, and J. V. Garcia. 1997. Induction of phosphorylation of human immunodeficiency virus type 1 nef and enhancement of CD4 downregulation by phorbol myristate acetate. J. Virol. 71:2535-2539[Abstract].
30.	MacDonald, T. T., and J. Spencer. 1994. Lymphoid cells and tissues of the gastrointestinal tract, p. 394-421. In R. H. Heatley (ed.), Gastrointestinal and hepatic immunology. Cambridge University Press, Cambridge, England
31.	Mahalingham, M., M. Peakman, E. T. Davies, A. Pozniak, T. J. McManus, and D. Vergani. 1993. T cell activation and disease severity in HIV infection. Clin. Exp. Immunol. 93:337-343[Medline].
32.	Malavasi, F., A. Funaro, S. Roggero, A. L. Horenstein, L. Calosso, and K. Mehta. 1994. Human CD38: one molecule in search of a function. Immunol. Today 15:95-97[CrossRef][Medline].
33.	McDougal, J. S., A. Mawle, S. P. Cort, J. K. A. Nicholson, G. D. Cross, J. A. Schleppler-Campbell, D. Hicks, and J. Sligh. 1985. Cellular tropism of the human retrovirus HTLV-III/LAV. I. Role of T cell activation and expression of the T4 antigen. J. Immunol. 135:3151-3162[Abstract].
34.	Mellors, J. W., C. R. Rinaldo, 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].
35.	Mowat, A. M., and J. L. Viney. 1997. The anatomical basis of intestinal immunity. Immunol. Rev. 156:145-166[CrossRef][Medline].
36.	Nabel, G., and D. Baltimore. 1987. An inducible transcription factor activates expression of human immunodeficiency virus in T cells. Nature 326:711-713[CrossRef][Medline].
37.	Orenstein, J. M., C. Fox, and S. M. Wahl. 1997. Macrophages as a source of HIV during opportunistic infections. Science 276:1857-1861[Abstract/Free Full Text].
38.	Pantaleo, G., C. Graziosi, and A. S. Fauci. 1997. Virologic and immunologic events in primary HIV infection. Springer Semin. Immunopathol. 18:257-266[CrossRef][Medline].
39.	Phillips, A. N. 1996. Reduction of HIV concentration during acute infection: independence from a specific immune response. Science 271:497-498[Abstract].
40.	Picker, L. J., J. R. Treer, B. Ferguson-Darnell, P. A. Collins, D. Buck, and L. W. M. M. Terstappen. 1993. Control of lymphocyte recirculation in man. 1. Differential regulation of the peripheral lymph node homing receptor L-selectin on T cells during the virgin to memory cell transition. J. Immunol. 150:1105-1121[Abstract].
41.	Piguet, V., and D. Trono. 1999. The nef protein of primate lentiviruses. Rev. Med. Virol. 9:111-120[CrossRef][Medline].
42.	Reinis, M., M. Morra, A. Funaro, R. Di Primio, and F. Malavasi. 1997. Functional associations of CD38 with CD3 on the T cell membrane. J. Biol. Regul. Homeost. Agents 11:137-142[Medline].
43.	Roederer, M., J. G. Dubs, M. T. Anderson, P. A. Raju, and L. A. Herzenberg. 1995. CD8 naive T cell counts decrease progressively in HIV-infected patients. J. Clin. Investig. 95:2061-2066.
44.	Sasseville, V. G., Z. Du, L. V. Chalifoux, D. R. Pauley, H. Y. Young, P. K. Sehgal, R. C. Desrosiers, and A. A. Lackner. 1996. Induction of lymphocyte proliferation and severe gastrointestinal disease in macaques by a nef gene variant of SIVmac239. Am. J. Pathol. 149:163-175[Abstract].
45.	Schmitz, J. E., M. J. Kuroda, S. Santra, V. G. Sasseville, M. A. Simon, M. A. Lifton, P. Racz, K. Tenner-Racz, M. Dalesandro, B. J. Scallon, J. Ghrayeb, M. A. Forman, D. C. Montefiori, E. P. Rieber, N. L. Letvin, and K. A. Reimann. 1999. Control of viremia in simian immunodeficiency virus infection by CD8+ lymphocytes. Science 283:857-860[Abstract/Free Full Text].
46.	Schneider, T., H.-U. Jahn, W. Schmidt, E.-O. Reicken, M. Zeitz, and R. Ulrich. 1995. Loss of CD4 T lymphocytes in patients infected with human immunodeficiency virus type 1 is more pronounced in the duodenal mucosa than in the peripheral blood. Gut 37:524-529[Abstract/Free Full Text].
47.	Schnittman, S. M., H. C. Lane, J. Greenhouse, J. S. Justement, M. Baseler, and A. S. Fauci. 1990. Preferential infection of CD4+ memory cells by human immunodeficiency virus type 1: evidence for a role in the selective T-cell functional defects observed in infected individuals. Proc. Natl. Acad. Sci. USA 87:6058-6062[Abstract/Free Full Text].
48.	Smit-McBride, Z., J. J. Mattapallil, M. McChesney, D. Ferrick, and S. Dandekar. 1998. Gastrointestinal T lymphocytes retain high potential for cytokine responses but have severe CD4⁺ T-cell depletion at all stages of simian immunodeficiency virus infection compared to peripheral lymphocytes. J. Virol. 72:6646-6656[Abstract/Free Full Text].
49.	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].
50.	Staprans, S. I., B. L. Hamilton, S. E. Follansbee, T. Elbeik, P. Barbosa, R. M. Grant, and M. B. Feinberg. 1995. Activation of virus replication after vaccination of HIV-1 infected individuals. J. Exp. Med. 182:1727-1737[Abstract/Free Full Text].
51.	van den Hove, L. E., P. Vandenberghe, S. W. Van Gool, J. L. Ceuppens, H. Demuynck, G. E. Verhoef, and M. A. Boogaerts. 1998. Peripheral blood lymphocyte subset shifts in patients with untreated hematological tumors: evidence for systemic activation of the T cell compartment. Leuk. Res. 22:175-184[CrossRef][Medline].
52.	van Noesel, C. J., R. A. Gruters, F. G. Terpstra, P. T. Schellekens, R. A. van Lier, and F. Miedema. 1990. Functional and phenotypic evidence for a selective loss of memory T cells in asymptomatic human immunodeficiency virus-infected men. J. Clin. Investig. 86:293-299.
53.	Veazey, R. S., M. DeMaria, L. V. Chalifoux, D. E. Shvetz, D. R. Pauley, H. L. Knight, M. Rosenzweig, R. P. Johnson, R. C. Desrosiers, and A. A. Lackner. 1998. Gastrointestinal tract as a major site of CD4+ T cell depletion and viral replication in SIV infection. Science 280:427-431[Abstract/Free Full Text].
54.	Veazey, R. S., and A. A. Lackner. 1998. The gastrointestinal tract and the pathogenesis of AIDS. AIDS 12:S35-S42.
55.	Veazey, R. S., M. Rosenzweig, D. E. Shvetz, D. R. Pauley, M. DeMaria, L. V. Chalifoux, R. P. Johnson, and A. A. Lackner. 1997. Characterization of gut-associated lymphoid tissues (GALT) of normal rhesus macaques. Clin. Immunol. Immunopathol. 82:230-242[CrossRef][Medline].
56.	Westmoreland, S. V., E. Halpern, and A. A. Lackner. 1998. Simian immunodeficiency virus encephalitis in rhesus macaques is associated with rapid disease progression. J. Neurovirol. 4:260-268[Medline].
57.	Whetter, L., F. J. Novembre, M. Saucier, S. Gummurulu, and S. Dewhurst. 1998. Costimulatory pathways in lymphocyte proliferation induced by the simian immunodeficiency virus SIVsmmPBj14. J. Virol. 72:6155-6158[Abstract/Free Full Text].
58.	Willerford, D. M., M. J. Gale, Jr., R. E. Benveniste, E. A. Clark, and W. M. Gallatin. 1990. Simian immunodeficiency virus is restricted to a subset of blood CD4+ T lymphocytes that includes memory cells. J. Immunol. 144:3779-3783[Abstract].
59.	Zeigler, S. F., F. Ramsdell, and M. R. Alderson. 1994. The activation antigen CD69. Stem Cells 12:456-465[Abstract].
60.	Zeitz, M., W. C. Greene, N. J. Peffer, and S. P. James. 1988. Lymphocytes isolated from the intestinal lamina propria of normal nonhuman primates have increased expression of genes associated with T cell activation. Gastroenterology 94:647-655[Medline].