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1. Parallel analysis of multiple human memory CD4+ T-cell subsets within antigen-specific responses using cell proliferation dyes

Author

Cook, L, Zaunders, J, Seddiki, N, van Bockel, D, Kelleher, AD, Munier, CML, Cook, L, Zaunders, J, Seddiki, N, van Bockel, D, Kelleher, AD, and Munier, CML

Abstract

Activation induced marker (AIM) assays are being used increasingly to measure antigen-specific T-cell responses, but this activation can alter cell lineage defining phenotypic markers. We aimed to extend the utility of AIM assays to enable pre-activation defined cell populations to be tracked and quantified within T-cell memory responses. We sorted three ex vivo CD4+ T-cell populations prior to any activation using well defined ex vivo lineage surface marker combinations. These populations were memory non-Tregs, CD39+ Tregs and CD39neg Tregs, although any three memory CD4+ T-cell populations able to be isolated by cell surface markers could potentially be tracked. These cells were labeled with three distinct fluorescent cell proliferation dyes (CFSE, CellTrace Violet and Cell Proliferation Dye eF670) and then all autologous PBMCs were reconstituted maintaining ex vivo cell ratios and CD25/OX40 AIM assays performed with CMV and HSV antigens. This approach enabled tracking of pre-defined cell populations within antigen stimulated responses using both activation marker and cell proliferation readouts. We confirmed that although CD39+ Tregs comprise a substantial proportion of AIM assay responses, they do not make substantial contributions to the proliferative response. This extends the utility of AIM assays to enable parallel analysis of the relative contribution of several CD4+ memory T-cell subsets to recall responses.

Published
2023

2. Layer-by-Layer Particles Deliver Epigenetic Silencing siRNA to HIV-1 Latent Reservoir Cell Types

Author

Czuba-Wojnilowicz, E, Klemm, V, Cortez-Jugo, C, Turville, S, Aggarwal, A, Caruso, F, Kelleher, AD, Ahlenstiel, CL, Czuba-Wojnilowicz, E, Klemm, V, Cortez-Jugo, C, Turville, S, Aggarwal, A, Caruso, F, Kelleher, AD, and Ahlenstiel, CL

Abstract

For over two decades, nanomaterials have been employed to facilitate intracellular delivery of small interfering RNA (siRNA), both in vitro and in vivo, to induce post-transcriptional gene silencing (PTGS) via RNA interference. Besides PTGS, siRNAs are also capable of transcriptional gene silencing (TGS) or epigenetic silencing, which targets the gene promoter in the nucleus and prevents transcription via repressive epigenetic modifications. However, silencing efficiency is hampered by poor intracellular and nuclear delivery. Here, polyarginine-terminated multilayered particles are reported as a versatile system for the delivery of TGS-inducing siRNA to potently suppress virus transcription in HIV-infected cells. siRNA is complexed with multilayered particles formed by layer-by-layer assembly of poly(styrenesulfonate) and poly(arginine) and incubated with HIV-infected cell types, including primary cells. Using deconvolution microscopy, uptake of fluorescently labeled siRNA is observed in the nuclei of HIV-1 infected cells. Viral RNA and protein are measured to confirm functional virus silencing from siRNA delivered using particles 16 days post-treatment. This work extends conventional particle-enabled PTGS siRNA delivery to the TGS pathway and paves the way for future studies on particle-delivered siRNA for efficient TGS of various diseases and infections, including HIV.

Published
2023

3. Tracking the clonal dynamics of SARS-CoV-2-specific T cells in children and adults with mild/asymptomatic COVID-19.

Author

Khoo, WH, Jackson, K, Phetsouphanh, C, Zaunders, JJ, Alquicira-Hernandez, J, Yazar, S, Ruiz-Diaz, S, Singh, M, Dhenni, R, Kyaw, W, Tea, F, Merheb, V, Lee, FXZ, Burrell, R, Howard-Jones, A, Koirala, A, Zhou, L, Yuksel, A, Catchpoole, DR, Lai, CL, Vitagliano, TL, Rouet, R, Christ, D, Tang, B, West, NP, George, S, Gerrard, J, Croucher, PI, Kelleher, AD, Goodnow, CG, Sprent, JD, Powell, JE, Brilot, F, Nanan, R, Hsu, PS, Deenick, EK, Britton, PN, Phan, TG, Khoo, WH, Jackson, K, Phetsouphanh, C, Zaunders, JJ, Alquicira-Hernandez, J, Yazar, S, Ruiz-Diaz, S, Singh, M, Dhenni, R, Kyaw, W, Tea, F, Merheb, V, Lee, FXZ, Burrell, R, Howard-Jones, A, Koirala, A, Zhou, L, Yuksel, A, Catchpoole, DR, Lai, CL, Vitagliano, TL, Rouet, R, Christ, D, Tang, B, West, NP, George, S, Gerrard, J, Croucher, PI, Kelleher, AD, Goodnow, CG, Sprent, JD, Powell, JE, Brilot, F, Nanan, R, Hsu, PS, Deenick, EK, Britton, PN, and Phan, TG

Abstract

Children infected with severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) develop less severe coronavirus disease 2019 (COVID-19) than adults. The mechanisms for the age-specific differences and the implications for infection-induced immunity are beginning to be uncovered. We show by longitudinal multimodal analysis that SARS-CoV-2 leaves a small footprint in the circulating T cell compartment in children with mild/asymptomatic COVID-19 compared to adult household contacts with the same disease severity who had more evidence of systemic T cell interferon activation, cytotoxicity and exhaustion. Children harbored diverse polyclonal SARS-CoV-2-specific naïve T cells whereas adults harbored clonally expanded SARS-CoV-2-specific memory T cells. A novel population of naïve interferon-activated T cells is expanded in acute COVID-19 and is recruited into the memory compartment during convalescence in adults but not children. This was associated with the development of robust CD4+ memory T cell responses in adults but not children. These data suggest that rapid clearance of SARS-CoV-2 in children may compromise their cellular immunity and ability to resist reinfection.

Published
2023

4. Early expansion of CD38+ICOS+ GC Tfh in draining lymph nodes during influenza vaccination immune response

Author

Law, H, Mach, M, Howe, A, Obeid, S, Milner, B, Carey, C, Elfis, M, Fsadni, B, Ognenovska, K, Phan, TG, Carey, D, Xu, Y, Venturi, V, Zaunders, J, Kelleher, AD, Munier, CML, Law, H, Mach, M, Howe, A, Obeid, S, Milner, B, Carey, C, Elfis, M, Fsadni, B, Ognenovska, K, Phan, TG, Carey, D, Xu, Y, Venturi, V, Zaunders, J, Kelleher, AD, and Munier, CML

Abstract

T follicular helper (Tfh) cells provide critical help to B cells during the germinal center (GC) reaction to facilitate generation of protective humoral immunity. Accessing the human lymph node (LN) to study the commitment of CD4 T cells to GC Tfh cell differentiation during in vivo vaccine responses is difficult. We used ultrasound guided fine needle biopsy to monitor recall responses in axillary LNs to seasonal influenza vaccination in healthy volunteers. Specific expansion of GC cell subsets occurred exclusively within draining LNs five days postvaccination. Draining LN GC Tfh and precursor-Tfh cells express higher levels of CD38, ICOS, and Ki67, indicating they were significantly more activated, motile, and proliferating, compared to contralateral LN cells. These observations provide insight into the early expansion phase of the human Tfh lineage within LNs during a vaccine induced memory response and highlights early LN immune responses may not be reflected in the periphery.

Published
2022

5. Nanoscale probing and imaging of HIV-1 RNA in cells with a chimeric LNA-DNA sensor

Author

Amodio, A, Cassani, M, Mummolo, L, Cortez-Jugo, C, Bhangu, SK, Symons, J, Ahlenstiel, CL, Forte, G, Ricci, F, Kelleher, AD, Lewin, SR, Cavalieri, F, Caruso, F, Amodio, A, Cassani, M, Mummolo, L, Cortez-Jugo, C, Bhangu, SK, Symons, J, Ahlenstiel, CL, Forte, G, Ricci, F, Kelleher, AD, Lewin, SR, Cavalieri, F, and Caruso, F

Abstract

Real-time detection and nanoscale imaging of human immunodeficiency virus type 1 ribonucleic acid (HIV-1 RNA) in latently infected cells that persist in people living with HIV-1 on antiretroviral therapy in blood and tissue may reveal new insights needed to cure HIV-1 infection. Herein, we develop a strategy combining DNA nanotechnology and super-resolution expansion microscopy (ExM) to detect and image a 22 base sequence transcribed from the HIV-1 promoter in model live and fixed cells. We engineer a chimeric locked nucleic acid (LNA)-DNA sensor via hybridization chain reaction to probe HIV-1 RNA in the U3 region of the HIV-1 long terminal repeat (LTR) by signal amplification in live cells. We find that the viral RNA transcript of the U3 region of the HIV-1 LTR, namely PromA, is a valid and specific biomarker to detect infected live cells. The efficiency and selectivity of the LNA-DNA sensor are evaluated in combination with ExM. Unlike standard ExM methods, which rely on additional custom linkers to anchor and immobilize RNA molecules in the intracellular polymeric network, in the current strategy, we probe and image the HIV-1 RNA target at nanoscale resolution, without resorting to chemical linkers or additional preparation steps. This is achieved by physical entrapment of the HIV-1 viral transcripts in the cells post-expansion by finely tuning the mesh size of the intracellular polymeric network.

Published
2022

6. Phenotypic and functional characteristics of highly differentiated CD57+NKG2C+ NK cells in HIV-1-infected individuals

Author

Kristensen, AB, Wragg, K, Vanderven, H, Lee, WS, Silvers, J, Kent, HE, Grant, MD, Kelleher, AD, Juno, JA, Kent, SJ, Parsons, MS, Kristensen, AB, Wragg, K, Vanderven, H, Lee, WS, Silvers, J, Kent, HE, Grant, MD, Kelleher, AD, Juno, JA, Kent, SJ, and Parsons, MS

Abstract

Natural killer (NK) cells are important anti-viral effector cells. The function and phenotype of the NK cells that constitute an individual's NK cell repertoire can be influenced by ongoing or previous viral infections. Indeed, infection with human cytomegalovirus (HCMV) drives the expansion of a highly differentiated NK cell population characterized by expression of CD57 and the activating NKG2C receptor. This NK cell population has also been noted to occur in HIV-1-infected individuals. We evaluated the NK cells of HIV-1-infected and HIV-1-uninfected individuals to determine the relative frequency of highly differentiated CD57+NKG2C+ NK cells and characterize these cells for their receptor expression and responsiveness to diverse stimuli. Highly differentiated CD57+NKG2C+ NK cells occurred at higher frequencies in HCMV-infected donors relative to HCMV-uninfected donors and were dramatically expanded in HIV-1/HCMV co-infected donors. The expanded CD57+NKG2C+ NK cell population in HIV-1-infected donors remained stable following antiretroviral therapy. CD57+NKG2C+ NK cells derived from HIV-1-infected individuals were robustly activated by antibody-dependent stimuli that contained anti-HIV-1 antibodies or therapeutic anti-CD20 antibody, and these NK cells mediated cytolysis through NKG2C. Lastly, CD57+NKG2C+ NK cells from HIV-1-infected donors were characterized by reduced expression of the inhibitory NKG2A receptor. The abundance of highly functional CD57+NKG2C+ NK cells in HIV-1-infected individuals raises the possibility that these NK cells could play a role in HIV-1 pathogenesis or serve as effector cells for therapeutic/cure strategies.

Published
2022

7. Nanoparticle Delivery Platforms for RNAi Therapeutics Targeting COVID-19 Disease in the Respiratory Tract.

Author

Zhang, Y, Almazi, JG, Ong, HX, Johansen, MD, Ledger, S, Traini, D, Hansbro, PM, Kelleher, AD, Ahlenstiel, CL, Zhang, Y, Almazi, JG, Ong, HX, Johansen, MD, Ledger, S, Traini, D, Hansbro, PM, Kelleher, AD, and Ahlenstiel, CL

Abstract

Since December 2019, a pandemic of COVID-19 disease, caused by the severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), has rapidly spread across the globe. At present, the Food and Drug Administration (FDA) has issued emergency approval for the use of some antiviral drugs. However, these drugs still have limitations in the specific treatment of COVID-19, and as such, new treatment strategies urgently need to be developed. RNA-interference-based gene therapy provides a tractable target for antiviral treatment. Ensuring cell-specific targeted delivery is important to the success of gene therapy. The use of nanoparticles (NPs) as carriers for the delivery of small interfering RNA (siRNAs) to specific tissues or organs of the human body could play a crucial role in the specific therapy of severe respiratory infections, such as COVID-19. In this review, we describe a variety of novel nanocarriers, such as lipid NPs, star polymer NPs, and glycogen NPs, and summarize the pre-clinical/clinical progress of these nanoparticle platforms in siRNA delivery. We also discuss the application of various NP-capsulated siRNA as therapeutics for SARS-CoV-2 infection, the challenges with targeting these therapeutics to local delivery in the lung, and various inhalation devices used for therapeutic administration. We also discuss currently available animal models that are used for preclinical assessment of RNA-interference-based gene therapy. Advances in this field have the potential for antiviral treatments of COVID-19 disease and could be adapted to treat a range of respiratory diseases.

Published
2022

8. CD73+ CD127high long-term memory CD4 T cells are highly proliferative in response to recall antigens and are early targets in hiv-1 infection

Author

Seddiki, N, Zaunders, J, Phetsouphanh, C, Brezar, V, Xu, Y, McGuire, HM, Bailey, M, McBride, K, Hey-Cunningham, W, Munier, CML, Cook, L, Kent, S, Lloyd, A, Cameron, B, De St Groth, BF, Koelsch, K, Danta, M, Hocini, H, Levy, Y, Kelleher, AD, Seddiki, N, Zaunders, J, Phetsouphanh, C, Brezar, V, Xu, Y, McGuire, HM, Bailey, M, McBride, K, Hey-Cunningham, W, Munier, CML, Cook, L, Kent, S, Lloyd, A, Cameron, B, De St Groth, BF, Koelsch, K, Danta, M, Hocini, H, Levy, Y, and Kelleher, AD

Abstract

HIV-1 infection rapidly leads to a loss of the proliferative response of memory CD4+ T lymphocytes, when cultured with recall antigens. We report here that CD73 expression defines a subset of resting memory CD4+ T cells in peripheral blood, which highly express the α-chain of the IL-7 receptor (CD127), but not CD38 or Ki-67, yet are highly proliferative in response to mitogen and recall antigens, and to IL-7, in vitro. These cells also preferentially express CCR5 and produce IL-2. We reasoned that CD73+ memory CD4+ T cells decrease very early in HIV-1 infection. Indeed, CD73+ memory CD4+ T cells comprised a median of 7.5% (interquartile range: 4.5–10.4%) of CD4+ T cells in peripheral blood from healthy adults, but were decreased in primary HIV-1 infection to a median of 3.7% (IQR: 2.6–6.4%; p = 0.002); and in chronic HIV-1 infection to 1.9% (IQR: 1.1–3%; p < 0.0001), and were not restored by antiretroviral therapy. Moreover, we found that a significant proportion of CD73+ memory CD4+ T cells were skewed to a gut-homing phenotype, expressing integrins α4 and β7, CXCR3, CCR6, CD161 and CD26. Accordingly, 20% of CD4+ T cells present in gut biopsies were CD73+. In HIV+ subjects, purified CD73+ resting memory CD4+ T cells in PBMC were infected with HIV-1 DNA, determined by real-time PCR, to the same level as for purified CD73-negative CD4+ T cells, both in untreated and treated subjects. Therefore, the proliferative CD73+ subset of memory CD4+ T cells is disproportionately reduced in HIV-1 infection, but, unexpectedly, their IL-7 dependent long-term resting phenotype suggests that residual infected cells in this subset may contribute significantly to the very long-lived HIV proviral DNA reservoir in treated subjects.

Published
2021

9. SARS-CoV-2 neutralizing antibodies: Longevity, breadth, and evasion by emerging viral variants

Author

Tea, F, Stella, AO, Aggarwal, A, Darley, DR, Pilli, D, Vitale, D, Merheb, V, Lee, FXZ, Cunningham, P, Walker, GJ, Fichter, C, Brown, DA, Rawlinson, WD, Isaacs, SR, Mathivanan, V, Hoffmann, M, Pöhlman, S, Mazigi, O, Christ, D, Rockett, RJ, Sintchenko, V, Hoad, VC, Irving, DO, Dore, GJ, Gosbell, IB, Kelleher, AD, Matthews, GV, Brilot, F, Turville, SG, Tea, F, Stella, AO, Aggarwal, A, Darley, DR, Pilli, D, Vitale, D, Merheb, V, Lee, FXZ, Cunningham, P, Walker, GJ, Fichter, C, Brown, DA, Rawlinson, WD, Isaacs, SR, Mathivanan, V, Hoffmann, M, Pöhlman, S, Mazigi, O, Christ, D, Rockett, RJ, Sintchenko, V, Hoad, VC, Irving, DO, Dore, GJ, Gosbell, IB, Kelleher, AD, Matthews, GV, Brilot, F, and Turville, SG

Abstract

The Severe Acute Respiratory Syndrome Coronavirus 2 (SAU ARS-CoV-2) antibody neutralization response and its evasion by emerging viral variants and variant of concern (VOC) are unknown, but critical to understand reinfection risk and breakthrough infection following vaccination. Antibody immunoreactivity against SARS-CoV-2 antigens and Spike variants, inhibition of Spike-driven virus–cell fusion, and infectious SARS-CoV-2 neutralization were characterized in 807 serial samples from 233 reverse transcription polymerase chain reaction (RT-PCR)–confirmed Coronavirus Disease 2019 (COVID-19) individuals with detailed demographics and followed up to 7 months. A broad and sustained polyantigenic immunoreactivity against SARS-CoV-2 Spike, Membrane, and Nucleocapsid proteins, along with high viral neutralization, was associated with COVID-19 severity. A subgroup of “high responders” maintained high neutralizing responses over time, representing ideal convalescent plasma donors. Antibodies generated against SARS-CoV-2 during the first COVID-19 wave had reduced immunoreactivity and neutralization potency to emerging Spike variants and VOC. Accurate monitoring of SARS-CoV-2 antibody responses would be essential for selection of optimal responders and vaccine monitoring and design.

Published
2021

10. Protective efficacy of the anti-HIV broadly neutralizing antibody PGT121 in the context of semen exposure

Author

Parsons, MS, Kristensen, AB, Selva, KJ, Lee, WS, Amarasena, T, Esterbauer, R, Wheatley, AK, Bavinton, BR, Kelleher, AD, Grulich, AE, Khoury, G, Juno, JA, Kent, SJ, Parsons, MS, Kristensen, AB, Selva, KJ, Lee, WS, Amarasena, T, Esterbauer, R, Wheatley, AK, Bavinton, BR, Kelleher, AD, Grulich, AE, Khoury, G, Juno, JA, and Kent, SJ

Abstract

Background: HIV-1 infections occur following viral exposure at anogenital mucosal surfaces in the presence of semen. Semen contains immunosuppressive and pro-inflammatory factors. Semen from HIV-1-infected donors contains anti-HIV-1 antibodies. We assessed if passively infused anti-HIV-1 neutralizing antibody conferred protection from rectal SHIVSF162P3 challenge at semen exposed mucosae. Methods: We pooled seminal plasma from HIV-1-infected donors. The pool was screened by ELISA for antibodies against HIV-1SF162 gp140. The ability of seminal plasma to inhibit macaque NK cells from responding to direct and antibody-dependent stimulation was assessed. The ability of seminal plasma to inhibit macaque granulocytes from mediating oxidative burst was also assessed. To demonstrate viral infectivity in the presence of seminal plasma, macaques (n = 4) were rectally challenged with SHIVSF162P3 following exposure to 2.5 mL of seminal plasma. To evaluate if anti-HIV-1 neutralizing antibody confers protection against rectal SHIV challenge at semen exposed mucosae, eight macaques were intravenously infused with PGT121, either wild type (n = 4) or the Fc receptor binding deficient LALA variant (n = 4), and rectally challenged with SHIVSF162P3 following exposure to 2.5 mL of seminal plasma. Findings: Anti-HIV-1SF162 gp140 antibodies were detected in seminal plasma. Seminal plasma inhibited direct and antibody-dependent NK cell activation and granulocyte oxidative burst in vitro. Rectal SHIVSF162P3 challenge of control macaques following seminal plasma exposure resulted in infection of all animals. All macaques infused with wild type or LALA PGT121 and challenged with SHIVSF162P3 following seminal plasma exposure were protected. Interpretation: PGT121 conferred protection against rectal SHIVSF162P3 challenge at semen exposed mucosae. Future research should investigate if semen alters protection conferred by antibodies more dependent on non-neutralizing functions.

Published
2021

11. Subtype-specific differences in transmission cluster dynamics of HIV-1 B and CRF01_AE in New South Wales, Australia

Author

Di Giallonardo, F, Pinto, AN, Keen, P, Shaik, A, Carrera, A, Salem, H, Selvey, C, Nigro, SJ, Fraser, N, Price, K, Holden, J, Lee, FJ, Dwyer, DE, Bavinton, BR, Geoghegan, JL, Grulich, AE, Kelleher, AD, Guy, R, Prestage, G, Zablotska, I, Duck, T, Cooper, C, Holt, M, de Wit, J, Kaldor, J, Wilson, D, Brotherton, A, Cooper, DA, Crooks, L, Whittaker, B, Callander, D, Madeddu, D, Schmidt, HM, Telfer, B, Boyd, M, McGill, S, Patel, P, Power, C, Pinto, A, Nigro, S, Gordon, T, Feeney, L, Bath, K, Mackie, B, Di Giallonardo, F, Pinto, AN, Keen, P, Shaik, A, Carrera, A, Salem, H, Selvey, C, Nigro, SJ, Fraser, N, Price, K, Holden, J, Lee, FJ, Dwyer, DE, Bavinton, BR, Geoghegan, JL, Grulich, AE, Kelleher, AD, Guy, R, Prestage, G, Zablotska, I, Duck, T, Cooper, C, Holt, M, de Wit, J, Kaldor, J, Wilson, D, Brotherton, A, Cooper, DA, Crooks, L, Whittaker, B, Callander, D, Madeddu, D, Schmidt, HM, Telfer, B, Boyd, M, McGill, S, Patel, P, Power, C, Pinto, A, Nigro, S, Gordon, T, Feeney, L, Bath, K, and Mackie, B

Abstract

Introduction: The human immunodeficiency virus 1 (HIV-1) pandemic is characterized by numerous distinct sub-epidemics (clusters) that continually fuel local transmission. The aims of this study were to identify active growing clusters, to understand which factors most influence the transmission dynamics, how these vary between different subtypes and how this information might contribute to effective public health responses. Methods: We used HIV-1 genomic sequence data linked to demographic factors that accounted for approximately 70% of all new HIV-1 notifications in New South Wales (NSW). We assessed differences in transmission cluster dynamics between subtype B and circulating recombinant form 01_AE (CRF01_AE). Separate phylogenetic trees were estimated using 2919 subtype B and 473 CRF01_AE sequences sampled between 2004 and 2018 in combination with global sequence data and NSW-specific clades were classified as clusters, pairs or singletons. Significant differences in demographics between subtypes were assessed with Chi-Square statistics. Results: We identified 104 subtype B and 11 CRF01_AE growing clusters containing a maximum of 29 and 11 sequences for subtype B and CRF01_AE respectively. We observed a > 2-fold increase in the number of NSW-specific CRF01_AE clades over time. Subtype B clusters were associated with individuals reporting men who have sex with men (MSM) as their transmission risk factor, being born in Australia, and being diagnosed during the early stage of infection (p < 0.01). CRF01_AE infections clusters were associated with infections among individuals diagnosed during the early stage of infection (p < 0.05) and CRF01_AE singletons were more likely to be from infections among individuals reporting heterosexual transmission (p < 0.05). We found six subtype B clusters with an above-average growth rate (>1.5 sequences / 6-months) and which consisted of a majority of infections among MSM. We also found four active growing CRF01_AE clusters contai

Published
2021

12. Altered Immune Reconstitution in Allogeneic Stem Cell Transplant Recipients with Human Immunodeficiency Virus (HIV)

Author

Murray, DD, Zaunders, J, Milliken, ST, Mee Ling Munier, C, Ford, C, Orla Morrissey, C, Visweswaran, M, Avery, S, Sasadeusz, J, Kwan, J, Desai, S, Law, M, Koelsch, KK, Lewin, SR, Moore, J, Kelleher, AD, Polizzotto, MN, Murray, DD, Zaunders, J, Milliken, ST, Mee Ling Munier, C, Ford, C, Orla Morrissey, C, Visweswaran, M, Avery, S, Sasadeusz, J, Kwan, J, Desai, S, Law, M, Koelsch, KK, Lewin, SR, Moore, J, Kelleher, AD, and Polizzotto, MN

Abstract

Background: Persons living with human immunodeficiency virus (HIV) are at elevated risk of developing the malignant diseases that require allogeneic stem cell transplantation (ASCT). Recent data suggest that these individuals are also at an elevated risk of certain complications post-ASCT. This risk may result from preexisting HIV-related factors affecting dynamics of immune reconstitution post-ASCT. However, to date, there has been little work describing the dynamics of immune reconstitution post-ASCT in persons with HIV and none comparing these data to controls without HIV. Methods: We assessed T-cell reconstitution in 6 ASCT with HIV recipients (HIV+ASCT) compared to a control population of 21 ASCT without HIV recipients. In a subset of HIV+ASCT recipients we performed additional flow cytometry profiling of CD8+ T-cell subsets and antigen specificity of reconstituting CD4+ and CD8+ T cells. Results: We observe no difference in post-ASCT CD4+ T cells between HIV+ASCT and HIV-negative ASCT recipients, despite much lower pre-ASCT CD4+ T-cell counts in the HIV+ASCT group. In contrast, we observed significantly higher CD8+ T-cell numbers in the HIV+ASCT group post-ASCT. The reconstituting CD8+ T-cells were predominantly CD45RO+, whereas homing markers and antigen specificity of these cells varied between participants. Conclusion: This study represents the most extensive characterization of immune-reconstitution post-ASCT in persons with HIV, and the first to our knowledge to compare these data to ASCT controls without HIV. The results indicate that immune reconstitution in this group can be affected by preexisting HIV infection and post-ASCT antigen exposure.

Published
2021

13. The role of zeb2 in human cd8 t lymphocytes: Clinical and cellular immune profiling in mowat–wilson syndrome

Author

Frith, K, Munier, CML, Hastings, L, Mowat, D, Wilson, M, Seddiki, N, Macintosh, R, Kelleher, AD, Gray, P, Zaunders, JJ, Frith, K, Munier, CML, Hastings, L, Mowat, D, Wilson, M, Seddiki, N, Macintosh, R, Kelleher, AD, Gray, P, and Zaunders, JJ

Abstract

The Zeb2 gene encodes a transcription factor (ZEB2) that acts as an important immune mediator in mice, where it is expressed in early‐activated effector CD8 T cells, and limits effector differentiation. Zeb2 homozygous knockout mice have deficits in CD8 T cells and NK cells. Mowat– Wilson syndrome (MWS) is a rare genetic disease resulting from heterozygous mutations in ZEB2 causing disease by haploinsufficiency. Whether ZEB2 exhibits similar expression patterns in human CD8 T cells is unknown, and MWS patients have not been comprehensively studied to identify changes in CD8 lymphocytes and NK cells, or manifestations of immunodeficiency. By using transcriptomic assessment, we demonstrated that ZEB2 is expressed in early‐activated effector CD8 T cells of healthy human volunteers following vaccinia inoculation and found evidence of a role for TGFß‐1/SMAD signaling in these cells. A broad immunological assessment of six genetically diagnosed MWS patients identified two patients with a history of recurrent sinopulmonary infections, one of whom had recurrent oral candidiasis, one with lymphopenia, two with thrombocytopenia and three with detectable anti‐nuclear antibodies. Immunoglobulin levels, including functional antibody responses to protein and polysaccharide vaccination, were normal. The MWS patients had a significantly lower CD8 T cell subset as % of lymphocytes, compared to healthy controls (median 16.4% vs. 25%, p = 0.0048), and resulting increased CD4:CD8 ratio (2.6 vs. 1.8; p = 0.038). CD8 T cells responded normally to mitogen stimulation in vitro and memory CD8 T cells exhibited normal proportions of subsets with important tissue‐specific homing markers and cytotoxic effector molecules. There was a trend towards a decrease in the CD8 T effector memory subset (3.3% vs. 5.9%; p = 0.19). NK cell subsets were normal. This is the first evidence that ZEB2 is expressed in early‐activated human effector CD8 T cells, and that haploinsufficiency of ZEB2 in MWS patients

Published
2021

14. SARS Coronavirus-2 Microneutralisation and Commercial Serological Assays Correlated Closely for Some but Not All Enzyme Immunoassays

Author

Walker, GJ, Naing, Z, Stella, AO, Yeang, M, Caguicla, J, Ramachandran, V, Isaacs, SR, Agapiou, D, Bull, RA, Stelzer-Braid, S, Daly, J, Gosbell, IB, Hoad, VC, Irving, DO, Pink, JM, Turville, S, Kelleher, AD, Rawlinson, WD, Walker, GJ, Naing, Z, Stella, AO, Yeang, M, Caguicla, J, Ramachandran, V, Isaacs, SR, Agapiou, D, Bull, RA, Stelzer-Braid, S, Daly, J, Gosbell, IB, Hoad, VC, Irving, DO, Pink, JM, Turville, S, Kelleher, AD, and Rawlinson, WD

Abstract

Serological testing for SARS-CoV-2-specific antibodies provides important research and diagnostic information relating to COVID-19 prevalence, incidence and host immune response. A greater understanding of the relationship between functionally neutralising antibodies detected using microneutralisation assays and binding antibodies detected using scalable enzyme immunoassays (EIA) is needed in order to address protective immunity post-infection or vaccination, and assess EIA suitability as a surrogate test for screening of convalescent plasma donors. We assessed whether neutralising antibody titres correlated with signal cut-off ratios in five commercially available EIAs, and one in-house assay based on expressed spike protein targets. Sera from recovered patients or convalescent plasma donors who reported laboratory-confirmed SARS-CoV-2 infection (n = 200), and negative control sera collected prior to the COVID-19 pandemic (n = 100), were assessed in parallel. Performance was assessed by calculating EIA sensitivity and specificity with reference to microneutralisation. Neutralising antibodies were detected in 166 (83%) samples. Compared with this, the most sensitive EIAs were the Cobas Elecsys Anti-SARS-CoV-2 (98%) and Vitros Immunodiagnostic Anti-SARS-CoV-2 (100%), which detect total antibody targeting the N and S1 antigens, respectively. The assay with the best quantitative relationship with microneutralisation was the Euroimmun IgG. These results suggest the marker used (total Ab vs. IgG vs. IgA) and the target antigen are important determinants of assay performance. The strong correlation between microneutralisation and some commercially available assays demonstrates their potential for clinical and research use in assessing protection following infection or vaccination, and use as a surrogate test to assess donor suitability for convalescent plasma donation.

Published
2021

15. A single dose, BCG-adjuvanted COVID-19 vaccine provides sterilising immunity against SARS-CoV-2 infection.

Author

Counoupas, C, Johansen, MD, Stella, AO, Nguyen, DH, Ferguson, AL, Aggarwal, A, Bhattacharyya, ND, Grey, A, Hutchings, O, Patel, K, Siddiquee, R, Stewart, EL, Feng, CG, Hansbro, NG, Palendira, U, Steain, MC, Saunders, BM, Low, JKK, Mackay, JP, Kelleher, AD, Britton, WJ, Turville, SG, Hansbro, PM, Triccas, JA, Counoupas, C, Johansen, MD, Stella, AO, Nguyen, DH, Ferguson, AL, Aggarwal, A, Bhattacharyya, ND, Grey, A, Hutchings, O, Patel, K, Siddiquee, R, Stewart, EL, Feng, CG, Hansbro, NG, Palendira, U, Steain, MC, Saunders, BM, Low, JKK, Mackay, JP, Kelleher, AD, Britton, WJ, Turville, SG, Hansbro, PM, and Triccas, JA

Abstract

Global control of COVID-19 requires broadly accessible vaccines that are effective against SARS-CoV-2 variants. In this report, we exploit the immunostimulatory properties of bacille Calmette-Guérin (BCG), the existing tuberculosis vaccine, to deliver a vaccination regimen with potent SARS-CoV-2-specific protective immunity. Combination of BCG with a stabilised, trimeric form of SARS-CoV-2 spike antigen promoted rapid development of virus-specific IgG antibodies in the blood of vaccinated mice, that was further augmented by the addition of alum. This vaccine formulation, BCG:CoVac, induced high-titre SARS-CoV-2 neutralising antibodies (NAbs) and Th1-biased cytokine release by vaccine-specific T cells, which correlated with the early emergence of T follicular helper cells in local lymph nodes and heightened levels of antigen-specific plasma B cells after vaccination. Vaccination of K18-hACE2 mice with a single dose of BCG:CoVac almost completely abrogated disease after SARS-CoV-2 challenge, with minimal inflammation and no detectable virus in the lungs of infected animals. Boosting BCG:CoVac-primed mice with a heterologous vaccine further increased SARS-CoV-2-specific antibody responses, which effectively neutralised B.1.1.7 and B.1.351 SARS-CoV-2 variants of concern. These findings demonstrate the potential for BCG-based vaccination to protect against major SARS-CoV-2 variants circulating globally.

Published
2021

16. Evaluation of commercially available viral transport medium (VTM) for SARS-CoV-2 inactivation and use in point-of-care (POC) testing

Author

Van Bockel, D, Munier, CML, Turville, S, Badman, SG, Walker, G, Stella, AO, Aggarwal, A, Yeang, M, Condylios, A, Kelleher, AD, Applegate, TL, Vallely, A, Whiley, D, Rawlinson, W, Cunningham, P, Kaldor, J, Guy, R, Van Bockel, D, Munier, CML, Turville, S, Badman, SG, Walker, G, Stella, AO, Aggarwal, A, Yeang, M, Condylios, A, Kelleher, AD, Applegate, TL, Vallely, A, Whiley, D, Rawlinson, W, Cunningham, P, Kaldor, J, and Guy, R

Abstract

Critical to facilitating SARS-CoV-2 point-of-care (POC) testing is assurance that viruses present in specimens are inactivated onsite prior to processing. Here, we conducted experiments to determine the virucidal activity of commercially available Viral Transport Mediums (VTMs) to inactivate SARS-CoV-2. Independent testing methods for viral inactivation testing were applied, including a previously described World Health Organization (WHO) protocol, in addition to a buffer exchange method where the virus is physically separated from the VTM post exposure. The latter method enables sensitive detection of viral viability at higher viral titre when incubated with VTM. We demonstrate that VTM formulations, Primestore® Molecular Transport Medium (MTM) and COPAN eNAT™ completely inactivate high-titre SARS-CoV-2 virus (>1 × 107 copies/mL) and are compatible with POC processing. Furthermore, full viral inactivation was rapidly achieved in as little as 2 min of VTM exposure. We conclude that adding certain VTM formulations as a first step post specimen collection will render SARS-CoV-2 non-infectious for transport, or for further in-field POC molecular testing using rapid turnaround GeneXpert platforms or equivalent.

Published
2020

17. Mucosal-associated invariant T (MAIT) cells are activated in the gastrointestinal tissue of patients with combination ipilimumab and nivolumab therapy-related colitis in a pathology distinct from ulcerative colitis

Author

Sasson, SC, Zaunders, JJ, Nahar, K, Munier, CML, Fairfax, BP, Olsson-Brown, A, Jolly, C, Read, SA, Ahlenstiel, G, Palendira, U, Scolyer, RA, Carlino, MS, Payne, MJ, Cheung, VTF, Gupta, T, Klenerman, P, Long, GV, Brain, O, Menzies, AM, Kelleher, AD, Sasson, SC, Zaunders, JJ, Nahar, K, Munier, CML, Fairfax, BP, Olsson-Brown, A, Jolly, C, Read, SA, Ahlenstiel, G, Palendira, U, Scolyer, RA, Carlino, MS, Payne, MJ, Cheung, VTF, Gupta, T, Klenerman, P, Long, GV, Brain, O, Menzies, AM, and Kelleher, AD

Abstract

The aim of this study was to investigate the pathogenesis of combination ipilimumab and nivolumab-associated colitis (IN-COL) by measuring gut-derived and peripheral blood mononuclear cell (GMNC; PBMC) profiles. We studied GMNC and PBMC from patients with IN-COL, IN-treated with no adverse-events (IN-NAE), ulcerative colitis (UC) and healthy volunteers using flow cytometry. In the gastrointestinal-derived cells we found high levels of activated CD8 T cells and mucosal-associated invariant T (MAIT) cells in IN-COL, changes that were not evident in IN-NAE or UC. UC, but not IN-C, was associated with a high proportion of regulatory T cells (T ). We sought to determine if local tissue responses could be measured in peripheral blood. Peripherally, checkpoint inhibition instigated a rise in activated memory CD4 and CD8 T cells, regardless of colitis. Low circulating MAIT cells at baseline was associated with IN-COL patients compared with IN-NAE in one of two cohorts. UC, but not IN-COL, was associated with high levels of circulating plasmablasts. In summary, the alterations in T cell subsets measured in IN-COL-affected tissue, characterized by high levels of activated CD8 T cells and MAIT cells and a low proportion of T , reflected a pathology distinct from UC. These tissue changes differed from the periphery, where T cell activation was a widespread on-treatment effect, and circulating MAIT cell count was low but not reliably predictive of colitis. + + + + reg reg

Published
2020

18. Increased hiv subtype diversity reflecting demographic changes in the hiv epidemic in new south wales, australia

Author

Di Giallonardo, F, Pinto, AN, Keen, P, Shaik, A, Carrera, A, Salem, H, Selvey, C, Nigro, SJ, Fraser, N, Price, K, Holden, J, Lee, FJ, Dwyer, DE, Bavinton, BR, Grulich, AE, Kelleher, AD, Di Giallonardo, F, Pinto, AN, Keen, P, Shaik, A, Carrera, A, Salem, H, Selvey, C, Nigro, SJ, Fraser, N, Price, K, Holden, J, Lee, FJ, Dwyer, DE, Bavinton, BR, Grulich, AE, and Kelleher, AD

Abstract

Changes over time in HIV-1 subtype diversity within a population reflect changes in factors influencing the development of local epidemics. Here we report on the genetic diversity of 2364 reverse transcriptase sequences from people living with HIV-1 in New South Wales (NSW) notified between 2004 and 2018. These data represent >70% of all new HIV-1 notifications in the state over this period. Phylogenetic analysis was performed to identify subtype-specific transmission clusters. Subtype B and non-B infections differed across all demographics analysed (p < 0.001). We found a strong positive association for infections among females, individuals not born in Australia or reporting heterosexual transmission being of non-B origin. Further, we found an overall increase in non-B infections among men who have sex with men from 50 to 79% in the last 10 years. However, we also found differences between non-B subtypes; heterosexual transmission was positively associated with subtype C only. In addition, the majority of subtype B infections were associated with clusters, while the majority of non-B infections were singletons. However, we found seven non-B clusters (≥5 sequences) indicative of local ongoing transmission. In conclusion, we present how the HIV-1 epidemic has changed over time in NSW, becoming more heterogeneous with distinct subtype-specific demographic associations.

Published
2020

19. Mapping the extent of heterogeneity of human CCR5R CD4R T cells in peripheral blood and lymph nodes

Author

Zaunders, J, Mee Ling Munier, C, McGuire, HM, Law, H, Howe, A, Xu, Y, De St Groth, BF, Schofield, P, Christ, D, Milner, B, Obeid, S, Dyer, WB, Saksena, NK, Kelleher, AD, Zaunders, J, Mee Ling Munier, C, McGuire, HM, Law, H, Howe, A, Xu, Y, De St Groth, BF, Schofield, P, Christ, D, Milner, B, Obeid, S, Dyer, WB, Saksena, NK, and Kelleher, AD

Abstract

Background: CD4 T cells that express the chemokine receptor, CCR5, are the most important target of HIV-1 infection, but their functions, phenotypes and anatomical locations are poorly understood. We aimed to use multiparameter flow cytometry to better define the full breadth of these cells. Methods: High-parameter fluorescence flow and mass cytometry were optimized to analyse subsets of CCR5 memory CD4 T cells, including CD25highCD127dim Tregs, CXCR3CCR6 Th1-like, CCR6CD161CXCR3 Th17-like, integrins a4ß7 guthoming, CCR4 skin-homing, CD62L lymph node-homing, CD38HLA-DR activated cells, and CD27CD28 cytotoxic T lymphocytes, in a total of 22 samples of peripheral blood, ultrasound-guided fine needle biopsies of lymph nodes and excised tonsils.CCR5 antigen-specific CD4 T cells were studied using the OX40 flow-based assay. Results: 10-20% of CCR5 memory CD4 T cells were Tregs, 10-30% were guthoming, 10-30% were skin-homing, 20-40% were lymph node-homing, 20-50% were Th1-like and 20-40% were Th17-like cells. Up to 30% were cytotoxic T lymphocytes in CMV-seropositive donors, including cells that were either CCR5high-Granzyme K or CCR5dimGranzyme B. When all possible phenotypes were exhaustively analysed, more than 150 different functional and trafficking subsets of CCR5 CD4 T cells were seen. Moreover, a small population of resident CD69Granzyme KCCR5 CD4 T cells was found in lymphoid tissues. CMV and Mycobacterium tuberculosis-specific CD4 T cells were predominantly CCR5. Conclusion: These results reveal for the first time the prodigious heterogeneity of function and trafficking of CCR5 CD4 T cells in blood and in lymphoid tissue, with significant implications for rational approaches to prophylaxis for HIV-1 infection and for purging of the HIV-1 reservoir in those participants already infected.

Published
2020

20. Mucosal IL-4R antagonist HIV vaccination with SOSIP-gp140 booster can induce high-quality cytotoxic CD4+/CD8+ T cells and humoral responses in macaques

Author

Li, Z, Khanna, M, Grimley, SL, Ellenberg, P, Gonelli, CA, Lee, WS, Amarasena, TH, Kelleher, AD, Purcell, DFJ, Kent, SJ, Ranasinghe, C, Li, Z, Khanna, M, Grimley, SL, Ellenberg, P, Gonelli, CA, Lee, WS, Amarasena, TH, Kelleher, AD, Purcell, DFJ, Kent, SJ, and Ranasinghe, C

Abstract

Inducing humoral, cellular and mucosal immunity is likely to improve the effectiveness of HIV-1 vaccine strategies. Here, we tested a vaccine regimen in pigtail macaques using an intranasal (i.n.) recombinant Fowl Pox Virus (FPV)-gag pol env-IL-4R antagonist prime, intramuscular (i.m.) recombinant Modified Vaccinia Ankara Virus (MVA)-gag pol-IL-4R antagonist boost followed by an i.m SOSIP-gp140 boost. The viral vector-expressed IL-4R antagonist transiently inhibited IL-4/IL-13 signalling at the vaccination site. The SOSIP booster not only induced gp140-specific IgG, ADCC (antibody-dependent cellular cytotoxicity) and some neutralisation activity, but also bolstered the HIV-specific cellular and humoral responses. Specifically, superior sustained systemic and mucosal HIV Gag-specific poly-functional/cytotoxic CD4+ and CD8+ T cells were detected with the IL-4R antagonist adjuvanted strategy compared to the unadjuvanted control. In the systemic compartment elevated Granzyme K expression was linked to CD4+ T cells, whilst Granzyme B/TIA-1 to CD8+ T cells. In contrast, the cytotoxic marker expression by mucosal CD4+ and CD8+ T cells differed according to the mucosal compartment. This vector-based mucosal IL-4R antagonist/SOSIP booster strategy, which promotes cytotoxic mucosal CD4+ T cells at the first line of defence, and cytotoxic CD4+ and CD8+ T cells plus functional antibodies in the blood, may prove valuable in combating mucosal infection with HIV-1 and warrants further investigation.

Published
2020

21. RNAi therapeutics: an antiviral strategy for human infections

Author

Kelleher, AD, Cortez-Jugo, C, Cavalieri, F, Qu, Y, Glanville, AR, Caruso, F, Symonds, G, Ahlenstiel, CL, Kelleher, AD, Cortez-Jugo, C, Cavalieri, F, Qu, Y, Glanville, AR, Caruso, F, Symonds, G, and Ahlenstiel, CL

Abstract

Gene silencing induced by RNAi represents a promising antiviral development strategy. This review will summarise the current state of RNAi therapeutics for treating acute and chronic human virus infections. The gene silencing pathways exploited by RNAi therapeutics will be described and include both classic RNAi, inducing cytoplasmic mRNA degradation post-transcription and novel RNAi, mediating epigenetic modifications at the transcription level in the nucleus. Finally, the challenge of delivering gene modifications via RNAi will be discussed, along with the unique characteristics of respiratory versus systemic administration routes to highlight recent advances and future potential of RNAi antiviral treatment strategies.

Published
2020

22. A single dose, BCG-adjuvanted COVID-19 vaccine provides sterilizing immunity against SARS-CoV-2 infection in mice

Author

Counoupas, C, Johansen, MD, Stella, AO, Nguyen, DH, Ferguson, AL, Aggarwal, A, Bhattacharyya, ND, Grey, A, Patel, K, Siddiquee, R, Stewart, EL, Feng, CG, Hansbro, NG, Palendira, U, Steain, MC, Saunders, BM, Low, JKK, Mackay, JP, Kelleher, AD, Britton, WJ, Turville, SG, Hansbro, PM, Triccas, JA, Counoupas, C, Johansen, MD, Stella, AO, Nguyen, DH, Ferguson, AL, Aggarwal, A, Bhattacharyya, ND, Grey, A, Patel, K, Siddiquee, R, Stewart, EL, Feng, CG, Hansbro, NG, Palendira, U, Steain, MC, Saunders, BM, Low, JKK, Mackay, JP, Kelleher, AD, Britton, WJ, Turville, SG, Hansbro, PM, and Triccas, JA

Published
2020

23. Possible clearance of transfusion-acquired nef/LTR-deleted attenuated HIV-1 infection by an elite controller with CCR5 Delta 32 heterozygous and HLA-B57 genotype

Author

Zaunders, J, Dyer, WB, Churchill, M, Munier, CML, Cunningham, PH, Suzuki, K, McBride, K, Hey-Nguyen, W, Koelsch, K, Wang, B, Hiener, B, Palmer, S, Gorry, PR, Bailey, M, Xu, Y, Danta, M, Seddiki, N, Cooper, DA, Saksena, NK, Sullivan, JS, Riminton, S, Learmont, J, Kelleher, AD, Zaunders, J, Dyer, WB, Churchill, M, Munier, CML, Cunningham, PH, Suzuki, K, McBride, K, Hey-Nguyen, W, Koelsch, K, Wang, B, Hiener, B, Palmer, S, Gorry, PR, Bailey, M, Xu, Y, Danta, M, Seddiki, N, Cooper, DA, Saksena, NK, Sullivan, JS, Riminton, S, Learmont, J, and Kelleher, AD

Abstract

Background: Subject C135 is one of the members of the Sydney Blood Bank Cohort, infected in 1981 through transfusion with attenuated nef/3′ long terminal repeat (LTR)-deleted HI V-1, and has maintained undetectable plasma viral load and steady CD4 cell count, in the absence of therapy. Uniquely, C135 combines five factors separately associated with control of viraemia: nef/LTR-deleted HI V-1, HLA -B57, HLA -DR13, heterozygous CCRccr5 Δ32 genotype and vigorous p24-stimulated peripheral blood mononuclear cell (PBMC) proliferation. Therefore, we studied in detail viral burden and immunological responses in this individual.Methods: PBMC and gut and lymph node biopsy samples were analysed for proviral HI V-1 DNA by real-time and nested PCR s, and nef/LTR alleles by nested PCR . HI V-specific antibodies were studied by Western blotting, and CD4+ and CD8+ T lymphocyte responses were measured by proliferation and cytokine production in vitro.Results: PBMC samples from 1996, but not since, showed amplification of nef alleles with gross deletions. Infectious HI V-1 was never recovered. Proviral HI V-1 DNA was not detected in recent PBMC or gut or lymph node biopsy samples. C135 has a consistently weak antibody response and a substantial CD4+ T cell proliferative response to a previously described HLA -DR13-restricted epitope of HI V-1 p24 in vitro, which augmented a CD8+ T cell response to an immunodominant HLA -B57-restricted epitope of p24, while his T cells show reduced levels of CCRccr5.Conclusions: Subject C135’s early PCR and weak antibody results are consistent with limited infection with a poorly replicating nef/LTR-deleted strain of HI V-1. With his HLA -B57-restricted gag-specific CD8 and helper HLA -DR13-restricted CD4 T cell proliferative responses, C135 appears to have cleared his HI V-1 infection 37 years after transfusion.

Published
2019

24. Functional cure of HIV: the scale of the challenge

Author

Davenport, MP, Khoury, DS, Cromer, D, Lewin, SR, Kelleher, AD, Kent, SJ, Davenport, MP, Khoury, DS, Cromer, D, Lewin, SR, Kelleher, AD, and Kent, SJ

Abstract

A variety of interventions to induce a functional cure of HIV are being explored, with the aim being to allow patients to cease antiretroviral therapy (ART) for prolonged periods of time or for life. These interventions share the goal of inducing ART-free remission from HIV pathogenesis and disease progression but achieve this in quite different ways, by reducing the size of the latent reservoir (for example, small-molecule stimulation of latently infected cells), reducing the number of target cells available for the virus (for example, gene therapy) or improving immune responses (for example, active or passive immunotherapy). Here, we consider a number of these alternative strategies for inducing post-treatment control of HIV and use mathematical modelling to predict the scale of the challenge inherent in these different approaches. For many approaches, over 99.9% efficacy will likely be required to induce durable ART-free remissions. The efficacy of individual approaches is currently far below what we predict will be necessary, and new technologies to achieve lifelong functional cure are needed.

Published
2019

25. HIV-1 DNA Is Maintained in Antigen-Specific CD4+ T Cell Subsets in Patients on Long-Term Antiretroviral Therapy Regardless of Recurrent Antigen Exposure

Author

Hey-Nguyen, WJ, Bailey, M, Xu, Y, Suzuki, K, Van Bockel, D, Finlayson, R, Leigh Brown, A, Carr, A, Cooper, DA, Kelleher, AD, Koelsch, KK, Zaunders, JJ, Hey-Nguyen, WJ, Bailey, M, Xu, Y, Suzuki, K, Van Bockel, D, Finlayson, R, Leigh Brown, A, Carr, A, Cooper, DA, Kelleher, AD, Koelsch, KK, and Zaunders, JJ

Abstract

Memory CD4+ T cells (mCD4s) containing integrated HIV DNA are considered the main barrier to a cure for HIV infection. Here, we analyzed HIV DNA reservoirs in antigen-specific subsets of mCDs to delineate the mechanisms by which HIV reservoirs persist during antiretroviral therapy (ART). HIV Gag, cytomegalovirus (CMV), and tetanus toxoid (TT)-specific mCD4s were isolated from peripheral blood samples obtained from 11 individual subjects, 2-11 years after commencing ART. Antigen-specific mCD4s were identified by the sensitive OX40 assay and purified by cell sorting. Total HIV DNA levels were quantified by real-time PCR, and clonal viral sequences generated from mCD4 subsets and pre-ART plasma samples. Quantitative results and sequence analysis were restricted to five and three study participants, respectively, which was likely due to the low frequency of the antigen-specific mCD4s and relatively low HIV DNA proviral loads. Median HIV Gag-, CMV-, and TT-specific mCD4s were 0.61%, 2.46%, and 0.78% of total mCD4s, and they contained a median of 2.50, 2.38, and 2.55 log 10 copies of HIV DNA per 10 6 cells, respectively. HIV DNA sequences were derived from antigen-specific mCD4s clustered with sequences derived from pre-ART plasma samples. There was a trend toward increased viral diversity in clonal viral sequences derived from CMV-specific mCD4s relative to TT-specific mCD4s. Despite limitations, this study provides direct evidence that HIV reservoirs persist in memory CD4+ T cell subsets maintained by homeostatic proliferation (TT) and adds to growing evidence against viral evolution during ART. Similar future studies require techniques that sample diverse HIV reservoirs and with improved sensitivity.

Published
2019

26. Limited sustained local transmission of HIV-1 CRF01_AE in New South Wales, Australia

Author

Di Giallonardo, F, Pinto, AN, Keen, P, Shaik, A, Carrera, A, Salem, H, Telfer, B, Cooper, C, Price, K, Selvey, C, Holden, J, Bachmann, N, Lee, FJ, Dwyer, DE, Duchêne, S, Holmes, EC, Grulich, AE, Kelleher, AD, Di Giallonardo, F, Pinto, AN, Keen, P, Shaik, A, Carrera, A, Salem, H, Telfer, B, Cooper, C, Price, K, Selvey, C, Holden, J, Bachmann, N, Lee, FJ, Dwyer, DE, Duchêne, S, Holmes, EC, Grulich, AE, and Kelleher, AD

Abstract

Australia’s response to the human immunodeficiency virus type 1 (HIV-1) pandemic led to effective control of HIV transmission and one of the world’s lowest HIV incidence rates—0.14%. Although there has been a recent decline in new HIV diagnoses in New South Wales (NSW), the most populous state in Australia, there has been a concomitant increase with non-B subtype infections, particularly for the HIV-1 circulating recombinant form CRF01_AE. This aforementioned CRF01_AE sampled in NSW, were combined with those sampled globally to identify NSW-specific viral clades. The population growth of these clades was assessed in two-year period intervals from 2009 to 2017. Overall, 109 NSW-specific clades were identified, most comprising pairs of sequences; however, five large clades comprising ≥10 sequences were also found. Forty-four clades grew over time with one or two sequences added to each in different two-year periods. Importantly, while 10 of these clades have seemingly discontinued, the remaining 34 were still active in 2016/2017. Seven such clades each comprised ≥10 sequences, and are representative of individual sub-epidemics in NSW. Thus, although the majority of new CRF01_AE infections were associated with small clades that rarely establish ongoing chains of local transmission, individual sub-epidemics are present and should be closely monitored.

Published
2019

27. Impact of HIV-1 viremia or sexually transmitted infection on semen-derived anti-HIV-1 antibodies and the immunosuppressive capacity of seminal plasma

Author

Selva, KJ, Bavinton, BR, Grulich, AE, Pazgier, M, Kelleher, AD, Kent, SJ, Parsons, MS, Selva, KJ, Bavinton, BR, Grulich, AE, Pazgier, M, Kelleher, AD, Kent, SJ, and Parsons, MS

Abstract

Semen from HIV-1-infected men contains anti-HIV-1 antibodies and immunosuppressive factor(s). We assessed if suppression of viremia with antiretroviral therapy impacted seminal plasma immunosuppressive capacity or the Fc-dependent functions of seminal anti-HIV-1 antibodies. We also tested if active bacterial sexually transmitted infections altered the immunosuppressive capacity of seminal plasma.

Published
2019

28. Mucosal and systemic SIV-specific cytotoxic CD4+ T cell hierarchy in protection following intranasal/intramuscular recombinant pox-viral vaccination of pigtail macaques

Author

Khanna, M, Jackson, RJ, Alcantara, S, Amarasena, TH, Li, Z, Kelleher, AD, Kent, SJ, Ranasinghe, C, Khanna, M, Jackson, RJ, Alcantara, S, Amarasena, TH, Li, Z, Kelleher, AD, Kent, SJ, and Ranasinghe, C

Abstract

A HIV vaccine that provides mucosal immunity is urgently needed. We evaluated an intranasal recombinant Fowlpox virus (rFPV) priming vaccine followed by intramuscular Modified Vaccinia Ankara (rMVA) booster vaccine, both expressing SIV antigens. The vaccination generated mucosal and systemic SIV-specific CD4+ T cell mediated immunity and was associated with partial protection against high-dose intrarectal SIVmac251 challenge in outbred pigtail macaques. Three of 12 vaccinees were completely protected and these animals elicited sustained Gag-specific poly-functional, cytotoxic mucosal CD4+ T cells, complemented by systemic poly-functional CD4+ and CD8+ T cell immunity. Humoral immune responses, albeit absent in completely protected macaques, were associated with partial control of viremia in animals with relatively weaker mucosal/systemic T cell responses. Co-expression of an IL-4R antagonist by the rFPV vaccine further enhanced the breadth and cytotoxicity/poly-functionality of mucosal vaccine-specific CD4+ T cells. Moreover, a single FPV-gag/pol/env prime was able to induce rapid anamnestic gp140 antibody response upon SIV encounter. Collectively, our data indicated that nasal vaccination was effective at inducing robust cervico-vaginal and rectal immunity, although cytotoxic CD4+ T cell mediated mucosal and systemic immunity correlated strongly with 'complete protection', the different degrees of protection observed was multi-factorial.

Published
2019

29. Memory B cells are reactivated in subcapsular proliferative foci of lymph nodes

Author

Moran, I, Nguyen, A, Khoo, WH, Butt, D, Bourne, K, Young, C, Hermes, JR, Biro, M, Gracie, G, Ma, CS, Munier, CML, Luciani, F, Zaunders, J, Parker, A, Kelleher, AD, Tangye, SG, Croucher, PI, Brink, R, Read, MN, Phan, TG, Moran, I, Nguyen, A, Khoo, WH, Butt, D, Bourne, K, Young, C, Hermes, JR, Biro, M, Gracie, G, Ma, CS, Munier, CML, Luciani, F, Zaunders, J, Parker, A, Kelleher, AD, Tangye, SG, Croucher, PI, Brink, R, Read, MN, and Phan, TG

Abstract

Vaccine-induced immunity depends on the generation of memory B cells (MBC). However, where and how MBCs are reactivated to make neutralising antibodies remain unknown. Here we show that MBCs are prepositioned in a subcapsular niche in lymph nodes where, upon reactivation by antigen, they rapidly proliferate and differentiate into antibody-secreting plasma cells in the subcapsular proliferative foci (SPF). This novel structure is enriched for signals provided by T follicular helper cells and antigen-presenting subcapsular sinus macrophages. Compared with contemporaneous secondary germinal centres, SPF have distinct single-cell molecular signature, cell migration pattern and plasma cell output. Moreover, SPF are found both in human and mouse lymph nodes, suggesting that they are conserved throughout mammalian evolution. Our data thus reveal that SPF is a seat of immunological memory that may be exploited to rapidly mobilise secondary antibody responses and improve vaccine efficacy.

Published
2018

30. Vorapaxar for HIV-associated inflammation and coagulopathy (ADVICE): a randomised, double-blind, placebo-controlled trial

Author

Kent, SJ, Hough, S, Kelleher, AD, Law, MG, Hutchinson, J, Catalfarmo, M, van Bockel, D, Lane, C, Baker, JV, Emery, S, Kent, SJ, Hough, S, Kelleher, AD, Law, MG, Hutchinson, J, Catalfarmo, M, van Bockel, D, Lane, C, Baker, JV, and Emery, S

Abstract

Background: Increased D-dimer concentrations are associated with poor cardiovascular and other clinical outcomes in people with treated HIV infection. Proteinase activated receptor-1 (PAR-1) is activated by thrombin and overexpressed by immune cells from HIV-infected people. We aimed to study the efficacy of vorapaxar, a licensed inhibitor of PAR-1, in reducing HIV-associated hypercoagulation and inflammation. Methods: This was a multicentre, double-blind, randomised, placebo-controlled trial done in seven hospital clinics in Australia and the USA. Eligible participants were HIV-infected, aviraemic, were receiving stable antiretroviral therapy, and had D-dimer concentrations greater than 200 ng/mL. We randomly assigned participants (1:1) using computer-generated block lists of size two to receive vorapaxar (2·5 mg orally daily) or matched placebo for 12 weeks. Participants were reviewed and had a blood sample taken at weeks 1, 4, 8, and 12 during treatment, and at a final visit at week 18. The primary endpoint was treatment group difference in changes from baseline D-dimer concentrations after 8–12 weeks of treatment, and was assessed in the modified intention-to-treat population (participants who had at least one dose of study drug or one follow-up visit). This trial is registered with ClinicalTrials.gov, number NCT02394730, and is closed to new participants. Findings: Between Oct 21, 2015, and July 14, 2017, 65 eligible patients were randomly assigned to the placebo group (n=31) or vorapaxar group (n=34). One patient from the vorapaxar group did not receive any study drug, and the modified intention-to-treat population was comprised of 33 patients. D-dimer concentrations after 8–12 weeks of treatment did not differ significantly between groups (difference −0·02 log10 ng/mL, 95% CI −0·10 to 0·05; p=0·56). Vorapaxar treatment was safe and well tolerated in this cohort. There were 161 adverse events (n=84 in the placebo group and n=77 in the vorapaxar group), and fiv

Published
2018

31. RNA-induced epigenetic silencing inhibits HIV-1 reactivation from latency

Author

Méndez, C, Ledger, S, Petoumenos, K, Ahlenstiel, C, Kelleher, AD, Méndez, C, Ledger, S, Petoumenos, K, Ahlenstiel, C, and Kelleher, AD

Abstract

Background: Current antiretroviral therapy is effective in controlling HIV-1 infection. However, cessation of therapy is associated with rapid return of viremia from the viral reservoir. Eradicating the HIV-1 reservoir has proven difficult with the limited success of latency reactivation strategies and reflects the complexity of HIV-1 latency. Consequently, there is a growing need for alternate strategies. Here we explore a "block and lock" approach for enforcing latency to render the provirus unable to restart transcription despite exposure to reactivation stimuli. Reactivation of transcription from latent HIV-1 proviruses can be epigenetically blocked using promoter-targeted shRNAs to prevent productive infection. We aimed to determine if independent and combined expression of shRNAs, PromA and 143, induce a repressive epigenetic profile that is sufficiently stable to protect latently infected cells from HIV-1 reactivation when treated with a range of latency reversing agents (LRAs). Results: J-Lat 9.2 cells, a model of HIV-1 latency, expressing shRNAs PromA, 143, PromA/143 or controls were treated with LRAs to evaluate protection from HIV-1 reactivation as determined by levels of GFP expression. Cells expressing shRNA PromA, 143, or both, showed robust resistance to viral reactivation by: TNF, SAHA, SAHA/TNF, Bryostatin/TNF, DZNep, and Chaetocin. Given the physiological importance of TNF, HIV-1 reactivation was induced by TNF (5 ng/mL) and ChIP assays were performed to detect changes in expression of epigenetic markers within chromatin in both sorted GFP - and GFP + cell populations, harboring latent or reactivated proviruses, respectively. Ordinary two-way ANOVA analysis used to identify interactions between shRNAs and chromatin marks associated with repressive or active chromatin in the integrated provirus revealed significant changes in the levels of H3K27me3, AGO1 and HDAC1 in the LTR, which correlated with the extent of reduced proviral reactivation. The cel

Published
2018

32. Divergent expression of CXCR5 and CCR5 on CD4+T cells and the paradoxical accumulation of T follicular helper cells during HIV infection

Author

Zaunders, J, Xu, Y, Kent, SJ, Koelsch, KK, Kelleher, AD, Zaunders, J, Xu, Y, Kent, SJ, Koelsch, KK, and Kelleher, AD

Abstract

© 2017 Zaunders, Xu, Kent, Koelsch and Kelleher. Viral infection sets in motion a cascade of immune responses, including both CXCR5+CD4+T follicular helper (Tfh) cells that regulate humoral immunity and CCR5+CD4+T cells that mediate cell-mediated immunity. In peripheral blood mononuclear cells, the majority of memory CD4+T cells appear to fall into either of these two lineages, CCR5-CXCR5+or CCR5+CXCR5-. Very high titers of anti-HIV IgG antibodies are a hallmark of infection, strongly suggesting that there is significant HIV-specific CD4+T cell help to HIV-specific B cells. We now know that characteristic increases in germinal centers (GC) in lymphoid tissue (LT) during SIV and HIV-1 infections are associated with an increase in CXCR5+PD-1highTfh, which expand to a large proportion of memory CD4+T cells in LT, and are presumably specific for SIV or HIV epitopes. Macaque Tfh normally express very little CCR5, yet are infected by CCR5-using SIV, which may occur mainly through infection of a subset of PD-1intermediateCCR5+Bcl-6+pre-Tfh cells. In contrast, in human LT, a subset of PD-1highTfh appears to express low levels of CCR5, as measured by flow cytometry, and this may also contribute to the high rate of infection of Tfh. Also, we have found, by assessing fine-needle biopsies of LT, that increases in Tfh and GC B cells in HIV infection are not completely normalized by antiretroviral therapy (ART), suggesting a possible long-lasting reservoir of infected Tfh. In contrast to the increase of CXCR5+Tfh, there is no accumulation of proliferating CCR5+CD4 T HIV Gag-specific cells in peripheral blood that make IFN-γ. Altogether, CXCR5+CCR5-CD4 T cells that regulate humoral immunity are allowed greater freedom to operate and expand during HIV-1 infection, but at the same time can contain HIV DNA at levels at least as high as in other CD4 subsets. We argue that early ART including a CCR5 blocker may directly reduce the infected Tfh reservoir in LT and also interrupt cycles

Published
2017

33. Differentiating founder and chronic HIV envelope sequences

Author

Murray, JM, Maher, S, Mota, T, Suzuki, K, Kelleher, AD, Center, RJ, Purcell, D, Murray, JM, Maher, S, Mota, T, Suzuki, K, Kelleher, AD, Center, RJ, and Purcell, D

Abstract

© 2017 Murray et al. This is an open access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited. Significant progress has been made in characterizing broadly neutralizing antibodies against the HIV envelope glycoprotein Env, but an effective vaccine has proven elusive. Vaccine development would be facilitated if common features of early founder virus required for transmission could be identified. Here we employ a combination of bioinformatic and operations research methods to determine the most prevalent features that distinguish 78 subtype B and 55 subtype C founder Env sequences from an equal number of chronic sequences. There were a number of equivalent optimal networks (based on the fewest covarying amino acid (AA) pairs or a measure of maximal covariance) that separated founders from chronics: 13 pairs for subtype B and 75 for subtype C. Every subtype B optimal solution contained the founder pairs 178-346 Asn-Val, 232-236 Thr-Ser, 240-340 Lys-Lys, 279-315 Asp-Lys, 291-792 Ala-Ile, 322-347 Asp-Thr, 535-620 Leu-Asp, 742-837 Arg- Phe, and 750-836 Asp-Ile; the most common optimal pairs for subtype C were 644-781 Lys-Ala (74 of 75 networks), 133-287 Ala-Gln (73/75) and 307-337 Ile-Gln (73/75). No pair was present in all optimal subtype C solutions highlighting the difficulty in targeting transmission with a single vaccine strain. Relative to the size of its domain (0.35% of Env), the α4β7 binding site occurred most frequently among optimal pairs, especially for subtype C: 4.2% of optimal pairs (1.2% for subtype B). Early sequences from 5 subtype B pre-seroconverters each exhibited at least one clone containing an optimal feature 553-624 (Ser-Asn), 724- 747 (Arg-Arg), or 46-293 (Arg-Glu).

Published
2017

34. HIV dynamics linked to memory CD4+ T cell homeostasis

Author

Murray, JM, Zaunders, J, Emery, S, Cooper, DA, Hey-Nguyen, WJ, Koelsch, KK, Kelleher, AD, Murray, JM, Zaunders, J, Emery, S, Cooper, DA, Hey-Nguyen, WJ, Koelsch, KK, and Kelleher, AD

Abstract

The dynamics of latent HIV is linked to infection and clearance of resting memory CD4+ T cells. Infection also resides within activated, non-dividing memory cells and can be impacted by antigen-driven and homeostatic proliferation despite suppressive antiretroviral therapy (ART). We investigated whether plasma viral level (pVL) and HIV DNA dynamics could be explained by HIV’s impact on memory CD4+ T cell homeostasis. Median total, 2-LTR and integrated HIV DNA levels per μL of peripheral blood, for 8 primary (PHI) and 8 chronic HIV infected (CHI) individuals enrolled on a raltegravir (RAL) based regimen, exhibited greatest changes over the 1st year of ART. Dynamics slowed over the following 2 years so that total HIV DNA levels were equivalent to reported values for individuals after 10 years of ART. The mathematical model reproduced the multiphasic dynamics of pVL, and levels of total, 2-LTR and integrated HIV DNA in both PHI and CHI over 3 years of ART. Under these simulations, residual viremia originated from reactivated latently infected cells where most of these cells arose from clonal expansion within the resting phenotype. Since virion production from clonally expanded cells will not be affected by antiretroviral drugs, simulations of ART intensification had little impact on pVL. HIV DNA decay over the first year of ART followed the loss of activated memory cells (120 day half-life) while the 5.9 year half-life of total HIV DNA after this point mirrored the slower decay of resting memory cells. Simulations had difficulty reproducing the fast early HIV DNA dynamics, including 2-LTR levels peaking at week 12, and the later slow loss of total and 2-LTR HIV DNA, suggesting some ongoing infection. In summary, our modelling indicates that much of the dynamical behavior of HIV can be explained by its impact on memory CD4+ T cell homeostasis.

Published
2017

35. Circulating MIR-122 and MIR-200a as biomarkers for fatal liver disease in ART-treated, HIV-1-infected individuals

Author

Murray, DD, Suzuki, K, Law, M, Trebicka, J, Neuhaus Nordwall, J, Johnson, M, Vjecha, MJ, Kelleher, AD, Emery, S, Murray, DD, Suzuki, K, Law, M, Trebicka, J, Neuhaus Nordwall, J, Johnson, M, Vjecha, MJ, Kelleher, AD, and Emery, S

Abstract

Liver disease is one of the main contributors to the increased levels of morbidity and mortality seen in the HIV-1-infected, ART-treated population. Circulating miRNAs, particularly those located inside extracellular vesicles, are seen as promising biomarkers for a number of human disease conditions, including liver-related diseases. Here, we show that serum levels of miR-122 and miR-200a are greater in HIV/HCV co-infected individuals compared to HIV-1 mono-infected individuals. We also show that miR-122 and miR-200a are elevated in ART-treated, HIV-1-infected individuals prior to the development of fatal liver disease, suggesting that these miRNA may have some potential clinical utility as biomarkers. While this study is hypothesis generating, it shows clearly that both miR-122 and miR-200a are promising novel biomarkers for liver disease in the ART-treated, HIV-1-infected population.

Published
2017

36. HIV-1 and SIV predominantly use CCR5 expressed on a precursor population to establish infection in T follicular helper cells

Author

Xu, Y, Phetsouphanh, C, Suzuki, K, Aggrawal, A, Graff-Dubois, S, Roche, M, Bailey, M, Alcantara, S, Cashin, K, Sivasubramaniam, R, Koelsch, KK, Autran, B, Harvey, R, Gorry, PR, Moris, A, Cooper, DA, Turville, S, Kent, SJ, Kelleher, AD, Zaunders, J, Xu, Y, Phetsouphanh, C, Suzuki, K, Aggrawal, A, Graff-Dubois, S, Roche, M, Bailey, M, Alcantara, S, Cashin, K, Sivasubramaniam, R, Koelsch, KK, Autran, B, Harvey, R, Gorry, PR, Moris, A, Cooper, DA, Turville, S, Kent, SJ, Kelleher, AD, and Zaunders, J

Abstract

© 2017 Xu, Phetsouphanh, Suzuki, Aggrawal, Graff-Dubois, Roche, Bailey, Alcantara, Cashin, Sivasubramaniam, Koelsch, Autran, Harvey, Gorry, Moris, Cooper, Turville, Kent, Kelleher and Zaunders. Background: T follicular helper (Tfh) cells are increasingly recognized as a major reservoir of HIV infection that will likely need to be addressed in approaches to curing HIV. However, Tfh express minimal CCR5, the major coreceptor for HIV-1, and the mechanism by which they are infected is unclear. We have previously shown that macaque Tfh lack CCR5, but are infected in vivo with CCR5-using SIV at levels comparable to other memory CD4+ T cells. Similarly, human splenic Tfh cells are highly infected with HIV-1 DNA. Therefore, we set out to examine the mechanism of infection of Tfh cells. Methodology: Tfh and other CD4+ T cell subsets from macaque lymph nodes and spleens, splenic Tfh from HIV+ subjects, and tonsillar Tfh from HIV-uninfected subjects were isolated by cell sorting prior to cell surface and molecular characterization. HIV proviral gp120 sequences were submitted to genotypic and phenotypic tropism assays. Entry of CCR5- and CXCR4-using viruses into Tfh from uninfected tonsillar tissue was measured using a fusion assay. Results: Phylogenetic analysis, genotypic, and phenotypic analysis showed that splenic Tfh cells from chronic HIV+ subjects were predominantly infected with CCR5-using viruses. In macaques, purified CCR5+PD-1intermediate(int)+ memory CD4+ T cells were shown to include pre-Tfh cells capable of differentiating in vitro to Tfh by upregulation of PD-1 and Bcl6, confirmed by qRT-PCR and single-cell multiplex PCR. Infected PD-1int cells survive, carry SIV provirus, and differentiate into PD-1hi Tfh after T cell receptor stimulation, suggesting a pathway for SIV infection of Tfh. In addition, a small subset of macaque and human PD-1hi Tfh can express low levels of CCR5, which makes them susceptible to infection. Fusion assays demonstrated CCR5-using HIV-1

Published
2017

37. Impact of Allogeneic Hematopoietic Stem Cell Transplantation on the HIV Reservoir and Immune Response in 3 HIV-Infected Individuals

Author

Koelsch, KK, Rasmussen, TA, Hey-Nguyen, WJ, Pearson, C, Xu, Y, Bailey, M, Marks, KH, Sasson, SC, Taylor, MS, Tantau, R, Obeid, S, Milner, B, Morrissey, O, Pinto, AN, Suzuki, K, Busch, MP, Keating, SM, Kaiser, P, Yukl, S, Wong, JK, Hiener, BM, Palmer, S, Zaunders, J, Post, JJ, Chan, DJ, Avery, S, Milliken, ST, Kelleher, AD, Lewin, SR, Cooper, DA, Koelsch, KK, Rasmussen, TA, Hey-Nguyen, WJ, Pearson, C, Xu, Y, Bailey, M, Marks, KH, Sasson, SC, Taylor, MS, Tantau, R, Obeid, S, Milner, B, Morrissey, O, Pinto, AN, Suzuki, K, Busch, MP, Keating, SM, Kaiser, P, Yukl, S, Wong, JK, Hiener, BM, Palmer, S, Zaunders, J, Post, JJ, Chan, DJ, Avery, S, Milliken, ST, Kelleher, AD, Lewin, SR, and Cooper, DA

Abstract

Background: Allogeneic hematopoietic stem cell transplantation (HSCT) can lead to significant changes to the HIV reservoir and HIV immune responses, indicating that further characterization of HIV-infected patients undergoing HSCT is warranted. Methods: We studied 3 patients who underwent HSCT after either reduced intensity conditioning or myeloablative conditioning regimen. We measured HIV antigens and antibodies (Ag/Ab), HIV-specific CD4 + T-cell responses, HIV RNA, and DNA in plasma, peripheral blood mononuclear cells, isolated CD4 + T cells from peripheral blood, and lymph node cells. The patients remained on antiretroviral therapy throughout the follow-up period. Results: All patients have been in continued remission for 4-6 years post-HSCT. Analyses of HIV RNA and DNA levels showed substantial reductions in HIV reservoir-related measurements in all 3 patients, changes in immune response varied with pronounced reductions in 2 patients and a less dramatic reduction in 1 patient. One patient experienced unexpected viral rebound 4 years after HSCT. Conclusions: These 3 cases highlight the substantial changes to the HIV reservoir and the HIV immune response in patients undergoing allogeneic HSCT. The viral rebound observed in 1 patient indicates that replication competent HIV can re-emerge several years after HSCT despite these marked changes.

Published
2017

38. Quantification of Residual Germinal Center Activity and HIV-1 DNA and RNA Levels Using Fine Needle Biopsies of Lymph Nodes during Antiretroviral Therapy

Author

Hey-Nguyen, WJ, Xu, Y, Pearson, CF, Bailey, M, Suzuki, K, Tantau, R, Obeid, S, Milner, B, Field, A, Carr, A, Bloch, M, Cooper, DA, Kelleher, AD, Zaunders, JJ, Koelsch, KK, Hey-Nguyen, WJ, Xu, Y, Pearson, CF, Bailey, M, Suzuki, K, Tantau, R, Obeid, S, Milner, B, Field, A, Carr, A, Bloch, M, Cooper, DA, Kelleher, AD, Zaunders, JJ, and Koelsch, KK

Abstract

HIV-1 reservoirs are most often studied in peripheral blood (PB), but not all lymphocytes recirculate, particularly T follicular helper (Tfh) CD4+ T cells, as well as germinal center (GC) B cells, in lymph nodes (LNs). Ultrasound-guided fine needle biopsies (FNBs) from inguinal LNs and PB samples were obtained from 10 healthy controls (HCs) and 21 HIV-1-infected subjects [11 antiretroviral therapy (ART) naive and 10 on ART]. Tfh cells and GC B cells were enumerated by flow cytometry. HIV-1 DNA and cell-associated (CA) RNA levels in LNs and PB were quantified by real-time polymerase chain reaction. FNBs were obtained without adverse events. Tfh cells and GC B cells were highly elevated in ART-naive subjects, with a median GC B cell count >300-fold higher than HCs, but also remained higher in 4 out of the 10 subjects on ART. GC B cell counts and Tfh cell counts were highly correlated with each other, and also with activated T cells in LNs but not in blood. Levels of HIV-1 DNA and CA RNA viral burden in highly purified CD4+ T cells from FNBs were significantly elevated compared with those in CD4+ T cells from PB in the ART-naive group, but only trended toward an increase in the ART patients. FNBs enabled minimally invasive access to, and parallel measurement of residual activated T and B cells and viral burden within LNs in HIV-1-infected patients. These FNBs revealed significant GC activity that was not apparent from corresponding PB samples.

Published
2017

39. Cytotoxic CD4 T Cells-Friend or Foe during Viral Infection?

Author

Juno, JA, van Bockel, D, Kent, SJ, Kelleher, AD, Zaunders, JJ, Munier, CML, Juno, JA, van Bockel, D, Kent, SJ, Kelleher, AD, Zaunders, JJ, and Munier, CML

Abstract

CD4 T cells with cytotoxic function were once thought to be an artifact due to long-term in vitro cultures but have in more recent years become accepted and reported in the literature in response to a number of viral infections. In this review, we focus on cytotoxic CD4 T cells in the context of human viral infections and in some infections that affect mice and non-human primates. We examine the effector mechanisms used by cytotoxic CD4 cells, the phenotypes that describe this population, and the transcription factors and pathways that lead to their induction following infection. We further consider the cells that are the predominant targets of this effector subset and describe the viral infections in which CD4 cytotoxic T lymphocytes have been shown to play a protective or pathologic role. Cytotoxic CD4 T cells are detected in the circulation at much higher levels than previously realized and are now recognized to have an important role in the immune response to viral infections.

Published
2017

40. Immune activation and immune aging in HIV infection

Author

Appay, V, Kelleher, AD, Appay, V, and Kelleher, AD

Abstract

Purpose of review The development of serious non-AIDS-related pathologies typically associated with aging, and the premature immune aging that characterizes HIV-1-infected patients, even with suppressive antiretroviral therapy, have raised increasing concerns in recent years. Deciphering the causes of these phenomena is key for our understanding of HIV pathogenesis and for the clinical care of patients living with the virus. Recent findings An important basis for the immune parallels between HIV infection and aging lies in the exhaustion of the lymphopoietic capacity of infected individuals, which eventually affects all compartments of the immune system. The alleged cause for these immune alterations, and the onset of age-related comorbidities, is the systemic chronic immune activation that is established in patients. However, there is a multiplicity of contributors to this immune activation. Summary Our understanding of the precise link between immune activation and aging in HIV infection is complicated by the influence of coinfections and life style factors. Developing rational interventions to reduce the hyper-inflammatory status of HIV-1-infected patients requires a clearer delineation of the factors contributing to the increased levels of systemic immune activation.

Published
2016

41. The feasibility of incorporating Vpx into lentiviral gene therapy vectors

Author

McAllery, SA, Ahlenstiel, CL, Suzuki, K, Symonds, GP, Kelleher, AD, Turville, SG, McAllery, SA, Ahlenstiel, CL, Suzuki, K, Symonds, GP, Kelleher, AD, and Turville, SG

Abstract

While current antiretroviral therapy has significantly improved, challenges still remain in life-long targeting of HIV-1 reservoirs. Lentiviral gene therapy has the potential to deliver protective genes into the HIV-1 reservoir. However, inefficient reverse transcription (RT) occurs in HIV-1 reservoirs during lentiviral gene delivery. The viral protein Vpx is capable of increasing lentiviral RT by antagonizing the restriction factor SAMHD1. Incorporating Vpx into lentiviral vectors could substantially increase gene delivery into the HIV-1 reservoir. The feasibility of this Vpx approach was tested in resting cell models utilizing macrophages and dendritic cells. Our results showed Vpx exposure led to increased permissiveness of cells over a period that exceeded 2 weeks. Consequently, significant lower potency of HIV-1 antiretrovirals inhibiting RT and integration was observed. When Vpx was incorporated with anti-HIV-1 genes inhibiting either pre-RT or post-RT stages of the viral life-cycle, transduction levels significantly increased. However, a stronger antiviral effect was only observed with constructs that inhibit pre-RT stages of the viral life cycle. In conclusion this study demonstrates a way to overcome the major delivery obstacle of gene delivery into HIV-1 reservoir cell types. Importantly, incorporating Vpx with pre-RT anti-HIV-1 genes, demonstrated the greatest protection against HIV-1 infection.

Published
2016

43. Correction: HIV Reactivation from Latency after Treatment Interruption Occurs on Average Every 5-8 Days-Implications for HIV Remission.

Author

Pinkevych, M, Cromer, D, Tolstrup, M, Grimm, AJ, Cooper, DA, Lewin, SR, Søgaard, OS, Rasmussen, TA, Kent, SJ, Kelleher, AD, Davenport, MP, Pinkevych, M, Cromer, D, Tolstrup, M, Grimm, AJ, Cooper, DA, Lewin, SR, Søgaard, OS, Rasmussen, TA, Kent, SJ, Kelleher, AD, and Davenport, MP

Abstract

[This corrects the article DOI: 10.1371/journal.ppat.1005000.][This corrects the article DOI: 10.1371/journal.ppat.1005740.][This corrects the article DOI: 10.1371/journal.ppat.1005679.].

Published
2016

46. Nuclear PKC-θ facilitates rapid transcriptional responses in human memory CD4+T cells through p65 and H2B phosphorylation

Author

Li, J, Hardy, K, Phetsouphanh, C, Tu, WJ, Sutcliffe, EL, McCuaig, R, Sutton, CR, Zafar, A, Mee Ling Munier, C, Zaunders, JJ, Xu, Y, Theodoratos, A, Tan, A, SiewLim, P, Knaute, T, Masch, A, Zerweck, J, Brezar, V, Milburn, PJ, Dunn, J, Casarotto, MG, Turner, SJ, Seddiki, N, Kelleher, AD, Rao, S, Li, J, Hardy, K, Phetsouphanh, C, Tu, WJ, Sutcliffe, EL, McCuaig, R, Sutton, CR, Zafar, A, Mee Ling Munier, C, Zaunders, JJ, Xu, Y, Theodoratos, A, Tan, A, SiewLim, P, Knaute, T, Masch, A, Zerweck, J, Brezar, V, Milburn, PJ, Dunn, J, Casarotto, MG, Turner, SJ, Seddiki, N, Kelleher, AD, and Rao, S

Abstract

MemoryTcells are characterizedby their rapid transcriptional programs upon re-stimulation. This transcriptional memory response is facilitated by permissive chromatin, but exactly how the permissive epigenetic landscape in memory T cells integrates incoming stimulatory signals remains poorly understood. By genome-wideChIP-sequencing ex vivo human CD4+T cells, here, we show that the signaling enzyme, protein kinase C theta (PKC-θ) directly relays stimulatory signals to chromatin by binding to transcriptional-memory-responsive genes to induce transcriptional activation. Flanked by permissive histone modifications, these PKC-enriched regions are significantly enriched with NF-κB motifs in ex vivo bulk and vaccinia-responsive human memory CD4+T cells. Within the nucleus, PKC-θ catalytic activity maintains the Ser536 phosphorylation on the p65 subunit of NF-κB (also known as RelA) and can directly influence chromatin accessibility at transcriptional memory genes by regulating H2B deposition through Ser32 phosphorylation. Furthermore, using a cytoplasm-restricted PKC-θ mutant, we highlight that chromatin-anchored PKC-θ integrates activating signals at the chromatin template to elicit transcriptional memory responses in human memory T cells.

Published
2016

47. The impact of transient combination antiretroviral treatment in early HIV infection on viral suppression and immunologic response in later treatment

Author

Pantazis, N, Touloumi, G, Meyer, L, Olson, A, Costagliola, D, Kelleher, AD, Lutsar, I, Chaix, ML, Fisher, M, Moreno, S, Porter, K, Pantazis, N, Touloumi, G, Meyer, L, Olson, A, Costagliola, D, Kelleher, AD, Lutsar, I, Chaix, ML, Fisher, M, Moreno, S, and Porter, K

Abstract

Objective: Effects of transient combination antiretroviral treatment (cART) initiated during early HIV infection (EHI) remain unclear. We investigate whether this intervention affects viral suppression and CD4+cell count increase following its reinitiation in chronic infection (CHI). Design: Longitudinal observational study. Methods: We identified adult patients from Concerted Action of Seroconversion to AIDS and Death in Europe who seroconverted after 1/1/2000, had a 12 months or less HIV test interval and initiated cART from naive. We classified individuals as 'pretreated in EHI' if treated within 6 months of seroconversion, interrupted for at least 12 weeks, and reinitiated during CHI. Statistical analysis was performed using survival analysis methods and mixed models. Results: Pretreated and initiated in CHI groups comprised 202 and 4263 individuals, with median follow-up after CHI treatment 4.5 and 3 years, respectively. Both groups had similar virologic response and relapse rates (P=0.585 and P=0.206) but pretreated individuals restarted treatment with higher baseline CD4+cell count (∼80cells/μl; P<0.001) and retained significantly higher CD4+cell count for more than 3 years after treatment (re)initiation. Assuming common baseline CD4+cell count, differences in CD4+cell count slopes were nonsignificant. Immunovirologic response to CHI treatment was not associated with timing or duration of the transient treatment. Conclusion: Although treatment interruptions are not recommended, stopping cART initiated in EHI does not seem to reduce the chance of a successful outcome of treatment in CHI.

Published
2016

48. Control of early HIV-1 infection associates with plasmacytoid dendritic cell-reactive opsonophagocytic IgG antibodies to HIV-1 p24

Author

Tjiam, MC, Sariputra, L, Armitage, JD, Taylor, JPA, Kelleher, AD, Tan, DBA, Lee, S, Fernandez, S, French, MA, Tjiam, MC, Sariputra, L, Armitage, JD, Taylor, JPA, Kelleher, AD, Tan, DBA, Lee, S, Fernandez, S, and French, MA

Abstract

Objectives: We have previously demonstrated that HIV-1 p24-specific plasmacytoid dendritic cell-reactive opsonophagocytic antibody (PROAb) responses associate with control of chronic HIV infection. Here, we examined whether HIV-1 p24-specific PROAbs associate with control of early HIV infection and their relationship with HIV-1 p24-specific IgG subclasses. Methods: Plasma collected at 8 and 52 weeks following primary HIV-1 infection was obtained from antiretroviral therapy-naïve patients who were classified as 'good' (plasma HIV-1 RNA<5000 copies/ml; n=17) or 'poor' (HIV-1 RNA>50 000 copies/ml; n=15) controllers at week 52. HIV-1 p24-specific PROAb responses were assayed using a plasmacytoid dendritic cell line (Gen2.2), and HIV-1 p24-specific IgG3, IgG1 and IgG2 levels were assayed by ELISA. Results: HIV-1 p24-specific PROAb responses increased in 'good controllers' (P=0.01) but remained unchanged in 'poor controllers' between weeks 8 and 52. Of the HIV-1 p24-specific IgG subclasses measured, only IgG1 increased over this time period in 'good controllers' alone (P=0.003), which correlated with the increase in HIV-1 p24-specific PROAb responses (r=0.83, P<0.0001). Depletion of IgG1 from IgG preparations of 'good controllers' resulted in the inhibition of HIV-1 p24-specific PROAb responses. In the total patient cohort, plasma HIV-1 RNA levels at week 52 correlated inversely with changes in HIV-1 p24-specific PROAb responses (r=-0.37, P=0.04) and IgG1 (r=-0.51, P=0.003) levels between weeks 8 and 52. Conclusion: Control of early HIV-1 infection was associated with an increase in HIV-1 p24-specific PROAb responses, which was mediated by HIV-1 p24-specific IgG1 antibodies. These findings provide further evidence that antibodies to HIV core proteins may contribute to control of HIV-1 infection.

Published
2016

49. CD4+ T follicular helper and IgA+ B cell numbers in gut biopsies from HIV-infected subjects on antiretroviral therapy are similar to HIV-uninfected individuals

Author

Zaunders, J, Danta, M, Bailey, M, Mak, G, Marks, K, Seddiki, N, Xu, Y, Templeton, DJ, Cooper, DA, Boyd, MA, Kelleher, AD, Koelsch, KK, Zaunders, J, Danta, M, Bailey, M, Mak, G, Marks, K, Seddiki, N, Xu, Y, Templeton, DJ, Cooper, DA, Boyd, MA, Kelleher, AD, and Koelsch, KK

Abstract

Background: Disruption of gastrointestinal tract epithelial and immune barriers contribute to microbial translocation, systemic inflammation, and progression of HIV-1 infection. Antiretroviral therapy (ART) may lead to reconstitution of CD4+ T cells in gut-associated lymphoid tissue (GALT), but its impact on humoral immunity within GALT is unclear. Therefore, we studied CD4+ subsets, including T follicular helper cells (Tfh), as well as resident B cells that have switched to IgA production, in gut biopsies, from HIV+ subjects on suppressive ART compared to HIV-negative controls (HNC). Methods: Twenty-three HIV+ subjects on ART and 22 HNC undergoing colonoscopy were recruited to the study. Single-cell suspensions were prepared from biopsies from left colon (LC), right colon (RC), and terminal ileum (TI). T and B lymphocyte subsets, as well as EpCAM+ epithelial cells, were accurately enumerated by flow cytometry, using counting beads. Results: No significant differences in the number of recovered epithelial cells were observed between the two subject groups. However, the median TI CD4+ T cell count/106 epithelial cells was 2.4-fold lower in HIV+ subjects versus HNC (19,679 versus 47,504 cells; p = 0.02). Similarly, median LC CD4+ T cell counts were reduced in HIV+ subjects (8,358 versus 18,577; p = 0.03) but were not reduced in RC. Importantly, we found no significant differences in Tfh or IgA+ B cell counts at either site between HIV+ subjects and HNC. Further analysis showed no difference in CD4+, Tfh, or IgA+ B cell counts between subjects who commenced ART in primary compared to chronic HIV-1 infection. Despite the decrease in total CD4 T cells, we could not identify a selective decrease of other key subsets of CD4+ T cells, including CCR5+ cells, CD127+ long-term memory cells, CD103+ tissue-resident cells, or CD161+ cells (surrogate marker for Th17), but there was a slight increase in the proportion of T regulatory cells. Conclusion: While there were lower absolu

Published
2016

50. Achieving HIV-1 Control through RNA-Directed Gene Regulation

Author

Klemm, V, Mitchell, J, Cortez-Jugo, C, Cavalieri, F, Symonds, G, Caruso, F, Kelleher, AD, Ahlenstiel, C, Klemm, V, Mitchell, J, Cortez-Jugo, C, Cavalieri, F, Symonds, G, Caruso, F, Kelleher, AD, and Ahlenstiel, C

Abstract

HIV-1 infection has been transformed by combined anti-retroviral therapy (ART), changing a universally fatal infection into a controllable infection. However, major obstacles for an HIV-1 cure exist. The HIV latent reservoir, which exists in resting CD4+ T cells, is not impacted by ART, and can reactivate when ART is interrupted or ceased. Additionally, multi-drug resistance can arise. One alternate approach to conventional HIV-1 drug treatment that is being explored involves gene therapies utilizing RNA-directed gene regulation. Commonly known as RNA interference (RNAi), short interfering RNA (siRNA) induce gene silencing in conserved biological pathways, which require a high degree of sequence specificity. This review will provide an overview of the silencing pathways, the current RNAi technologies being developed for HIV-1 gene therapy, current clinical trials, and the challenges faced in progressing these treatments into clinical trials.

Published
2016

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