Back to results

Reversing Tissue Fibrosis to Improve Immune Reconstitution in HIV

Primary Purpose

HIV Infection, HIV Infections

Status

Completed

Phase

Phase 2

Locations

United States

Study Type

Interventional

Intervention

Losartan

Placebo

About this trial

This is an interventional treatment trial for HIV Infection focused on measuring Infection, HIV 1, HIV, Losartan, Fibrosis, Immune Activation, Immune Reconstitution

Eligibility Criteria

18 Years - undefined (Adult, Older Adult)All SexesAccepts Healthy Volunteers

HIV infected participants:

Inclusion Criteria:
Participants must meet all of the following inclusion criteria to participate in this study:
- HIV-1 infected.
  -≥ 18 years of age.
- Baseline peripheral CD4+ T cell count 200-600 cells/mm3 for at least two measures over the 6 months prior to study enrollment.
  -≥ 12 months of stable ART, defined as use of a given drug regimen without disruption lasting ≥ 1 week in the period leading up to study enrollment.
- HIV viral load (VL) < 50 copies/mL for at least two consecutive measures over the 6 months prior to study enrollment.
- No contraindication to proposed study procedures.
- Women of child-bearing potential must be willing to use a form of effective contraception for the duration of the study. Effective contraception includes hormonal injection, implant or oral medication, IUD, diaphragm, or cervical cap with spermicide. Condoms cannot be used as the sole form of contraception.
Exclusion Criteria: Participants meeting any of the following exclusion criteria at baseline will be excluded from study participation:
- Use of any immunomodulator within the 12 months prior to study enrollment. An immunomodulator for the purposes of this study is defined as a drug known to either diminish or augment a patient's immune system. Examples of these include, but are not limited to, systemic corticosteroids (use of topical steroids will be permitted), TNF-inhibitors, rituximab, cyclophosphamide, abatacept,cyclosporine, azathioprine, 6-mercaptopurine, methotrexate, sulfasalazine, cyclosporine, tacrolimus,sirolimus, and intravenous immune globulin.
- Current use of an ARB or ACEi.
- Current use of rifaximin, fluconazole or lithium given potential for drug interactions with losartan.
- Prior reaction or intolerance to an ARB or ACEi.
- Prior diagnosis of a chronic inflammatory disease with serologic or clinical evidence as diagnosed by a primary care physician or specialist. Examples of these include, but are not limited to, systemic lupus erythematosus, rheumatoid arthritis, scleroderma, Sjogren's syndrome, mixed connective tissue disease, psoriasis, polymyositis, dermatomyositis, vasculitis, sarcoidosis, Wegener's granulomatosis, giant cell arteritis, polyarteritis nodosa, gastrointestinal pemphigoid, eosinophilic colitis, Crohn's disease, ulcerative colitis, autoimmune hepatitis, and hepatitis C.
- Prior diagnosis of a connective tissue disease with genetic, serologic or clinical evidence as diagnosed by a primary care physician or specialist (Marfan's syndrome, Ehlers-Danlos syndrome).
- Baseline blood pressure < 110/70.
- Estimated Glomerular Filtration Rate (eGFR) of < 30ml/min/1.73 m2 within 4 weeks of study initiation or history of advanced renal disease.
- AST and/or ALT > 3 times the upper limit of normal within 4 weeks of study enrollment.
- Potassium > 5.0 within 4 weeks of study enrollment.
- Pregnancy.
- In women of childbearing age, unwillingness to use birth control for the duration of the study.
- Breast feeding.
- Prior vaccination with an HPV vaccine, including Cervarix (GlaxoSmithKline) or Gardasil (Merck).
- History of hypersensitivity or severe allergic reactions to yeast.

HIV-uninfected:

Inclusion Criteria
Participants must meet all of the following inclusion criteria to participate in this study:
- HIV uninfected.
  -≥ 18 years of age.
- No contraindication to proposed study procedures.
Exclusion Criteria: Participants meeting any of the following exclusion criteria at baseline will be excluded from study participation:
- Use of any immunomodulator within the 12 months prior to study enrollment (as defined above).
- Current use of an ARB or ACEi.
- Prior diagnosis of a chronic inflammatory disease with serologic or clinical evidence (as defined above).
- Prior diagnosis of a connective tissue disease with genetic, serologic or clinical evidence as diagnosed by a primary care physician or specialist (Marfan's syndrome, Ehlers-Danlos syndrome).
- Pregnancy.

Sites / Locations

University of Minnesota, Division of Infectious Diseases

Arms of the Study

Arm 1

Arm 2

Arm Type

Experimental

Placebo Comparator

Arm Label

Losartan

Sugar Pill

Arm Description

Outcomes

Primary Outcome Measures

Collagen Deposition in LT

The Impact of Losartan Treatment on Lymphoid Tissue (LT) Fibrosis will be determined by measuring the amount of collagen deposition in LT using immunohistochemistry (IHC) and quantitative image analysis (QIA). LT will be obtained at baseline, month 12 and month 30.

Integrity of the Fibroblastic Reticular Cell Network (FRCn)

The Impact of Losartan Treatment on Lymphoid Tissue (LT) Fibrosis will be determined by measuring the Integrity of the fibroblastic reticular cell network (FRCn) using immunohistochemistry (IHC) and quantitative image analysis (QIA). LT will be obtained at baseline, month 12 and month 30.

Secondary Outcome Measures

Frequency of CD4+ T Cells

Impact of losartan on immune reconstitution and function will be determined by frequency of CD4+ T cells in LT using IHC.

Frequency TUNEL+CD3+CD8+ T Cells

Impact of losartan on immune reconstitution and function will be determined by frequency of TUNEL+CD3+CD8+ T cells in LT using IHC.

Frequency of Cells Expressing TGF-beta and Lymphotoxin-beta

Impact of losartan on immune reconstitution and function will be determined by frequency of cells expressing TGF-beta and lymphotoxin-beta in LT using IHC.

Serum Concentration of IL-7

Impact of losartan on immune reconstitution and function will be determine by serum concentrations of IL-7 measured with ELISA.

Serum Concentration of TGF-beta

Impact of losartan on immune reconstitution and function will be determine by serum concentrations of TGF-beta measured with ELISA.

Immune Response to HPV Vaccination

Impact of losartan on immune reconstitution and function will be determine by measuring the immune response to HPV vaccination using flow cytometry to identify cells stimulated by specific HPV peptides.

Frequency of Activated T-cell Populations - Immunofluorescent Staining

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the frequency of activated T-cell populations (specifically CD3+CD4+CD38+, CD3+,CD8+CD38+,CD4+Ki67+ and CD8+Ki67+ T cells) in LT using immunofluorescence staining

Percent of Activated T Cells in PBMCs - Flow Cytometry

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the percentage of activated T cells in peripheral blood mononuclear cells (PBMCs) using flow cytometry.

Percent of Activated Macrophages in PBMCs - Flow Cytometry

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the percentage of activated macrophages in peripheral blood mononuclear cells (PBMCs) using flow cytometry.

Percent of Activated Dendritic Cells in PBMCs - Flow Cytometry

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the percentage of activated dendritic cells in peripheral blood mononuclear cells (PBMCs) using flow cytometry.

Percent of Activated T Cells in LT - Flow Cytometry

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the percentage of activated T cells in lymphoid tissues (LT) using flow cytometry.

Percent of Activated Macrophages in LT - Flow Cytometry

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the percentage of activated macrophages in lymphoid tissues (LT) using flow cytometry.

Percent of Activated Dendritic Cells in LT - Flow Cytometry

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the percentage of activated dendritic cells in lymphoid tissues (LT) using flow cytometry.

Intracellular Concentration of IL-17 in PBMCs

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the intracellular levels of the inflammatory cytokine IL-17 in PBMCs using cytokine staining.

Intracellular Concentration of IFNg in PBMCs

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the intracellular levels of the inflammatory cytokine IFNg in PBMCs using cytokine staining.

Intracellular Concentration of IL-2 in PBMCs

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the intracellular levels of the inflammatory cytokine IL-2 in PBMCs using cytokine staining.

Intracellular Concentration of TNF in PBMCs

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the intracellular levels of the inflammatory cytokine TNF in PBMCs using cytokine staining.

Intracellular Concentration of IL-10 in PBMCs

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the intracellular levels of the inflammatory cytokine IL-10 in PBMCs using cytokine staining.

Intracellular Concentration of GM-CSF in PBMCs

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the intracellular levels of the inflammatory cytokine GM-CSF in PBMCs using cytokine staining.

Intracellular Concentration of IL-17 in LT

Intracellular Concentration of IFNg in LT

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the intracellular levels of the inflammatory cytokine IFNg in lymphoid tissue (LT) using cytokine staining.

Intracellular Concentration of IL-2 in LT

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the intracellular levels of the inflammatory cytokine IL-2 in lymphoid tissue (LT) using cytokine staining.

Intracellular Concentration of TNF in LT

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the intracellular levels of the inflammatory cytokine TNF in lymphoid tissue (LT) using cytokine staining.

Intracellular Concentration of IL-10 in LT

Intracellular Concentration of GM-CSF in LT

Plasma Concentration of LPS

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of LPS by ELISA.

Plasma Concentration of sCD14

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of sCD14 by limulus assay.

Plasma Concentration of I-FABP

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of I-FABP using ELISA.

Plasma Concentration of IL-1b

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of IL-1b using ELISA.

Plasma Concentration of IL-1RA

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of IL-1RA using ELISA.

Plasma Concentration of IL-6

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of IL-6 using ELISA.

Plasma Concentration of TNF

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of TNF using ELISA.

Plasma Concentration of Amyloid A

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of amyloid A using ELISA.

Plasma Concentration of CRP

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of CRP using ELISA.

Plasma Concentration of D-dimer

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of D-dimer using ELISA.

Frequency of HIV RNA+ and DNA+ Cells in LN - Radiolabeled ISH

The Potential for Losartan to Reduce the Size of the Viral Reservoir will be assessed by determining the frequency of HIV RNA+ and DNA+ cells in LN using radiolabeled in situ hybridization (ISH).

Frequency of HIV RNA+ and DNA+ Cells in LN - RNAscopeTM in Situ Technology

The Potential for Losartan to Reduce the Size of the Viral Reservoir will be assessed by determining the frequency of HIV RNA+ and DNA+ cells in LN using RNAscopeTM in situ technology.

Frequency of HIV RNA+ and DNA+ Cells in GALT - Radiolabeled in Situ Hybridization (ISH)

The Potential for Losartan to Reduce the Size of the Viral Reservoir will be assessed by determining the frequency of HIV RNA+ and DNA+ cells in GALT radiolabeled in situ hybridization (ISH).

Frequency of HIV RNA+ and DNA+ Cells in GALT - RNAscopeTM in Situ Technology

The Potential for Losartan to Reduce the Size of the Viral Reservoir will be assessed by determining the frequency of HIV RNA+ and DNA+ cells in GALT using RNAscopeTM in situ technology.

Concentration of Losartan and Antiretrovirals (ARVs)

Potential Drug-drug Interactions Between Losartan and Antiretrovirals (ARVs) will be assessed by measuring levels of ARVs and losartan in plasma and peripheral blood mononuclear cells (PBMCs).

Intracellular Concentration of Losartan and Antiretrovirals (ARVs)

Potential Drug-drug Interactions Between Losartan and Antiretrovirals (ARVs) will be assessed by measuring intracellular concentration of losartan and ARVs in lympoidtissue.

Full Information

NCT ID

NCT01852942

First Posted

February 20, 2012

Last Updated

November 16, 2020

Sponsor

University of Minnesota

Collaborators

National Institute of Allergy and Infectious Diseases (NIAID), Merck Sharp & Dohme LLC

1. Study Identification

Unique Protocol Identification Number

NCT01852942

Brief Title

Reversing Tissue Fibrosis to Improve Immune Reconstitution in HIV

Official Title

Reversing Tissue Fibrosis to Improve Immune Reconstitution in HIV

Study Type

Interventional

2. Study Status

Record Verification Date

November 2020

Overall Recruitment Status

Completed

Study Start Date

September 2014 (Actual)

Primary Completion Date

July 16, 2019 (Actual)

Study Completion Date

July 16, 2019 (Actual)

3. Sponsor/Collaborators

Responsible Party, by Official Title

Sponsor

Name of the Sponsor

University of Minnesota

Collaborators

National Institute of Allergy and Infectious Diseases (NIAID), Merck Sharp & Dohme LLC

4. Oversight

Data Monitoring Committee

Yes

5. Study Description

Brief Summary

This study was designed to test the hypothesis that treatment of HIV infected subjects with losartan, an agent with specific anti-inflammatory and anti-fibrotic actions, will: reverse existing lymphoid tissue fibrosis, restore lymphoid tissue architecture, increase the number and improve the function of peripheral and lymphatic CD4 T cells, decrease levels of systemic immune activation (IA), decrease size of the HIV reservoir, and be safe and well tolerated.

Detailed Description

This is a randomized, double-blind, placebo-controlled trial of 50 HIV-1 infected individuals on stable ART randomized in a 1:1 ratio to losartan (50 mg orally daily titrated to 100 mg daily) vs placebo for 30 months. We plan to enroll a total of 63 HIV infected subjects to ensure that 50 complete the protocol. All HIV infected subjects will undergo biopsies of inguinal lymph node (LN) and gut associated lymphatic tissue (GALT) for primary endpoint analysis at baseline, 12 and 30 months after study enrollment. Blood will be collected at least quarterly throughout the study and an intensive blood pharmacokinetic (PK) study will be conducted at month 1. All HIV infected subjects will be vaccinated with the quadrivalent human papillomavirus (HPV) vaccine at months 23, 25 and 29.5 to measure immune function. 5 HIV uninfected control subjects will also be enrolled. The primary endpoint is to determine the impact of losartan on lymphoid tissue fibrosis in HIV infected, ART treated adults. This will be determined by measuring the amount of collagen deposition in lymphoid tissues and the integrity of the FRCn using immunohistochemistry (IHC) and quantitative image analysis (QIA).

6. Conditions and Keywords

Primary Disease or Condition Being Studied in the Trial, or the Focus of the Study

HIV Infection, HIV Infections

Keywords

Infection, HIV 1, HIV, Losartan, Fibrosis, Immune Activation, Immune Reconstitution

7. Study Design

Primary Purpose

Treatment

Study Phase

Phase 2

Interventional Study Model

Parallel Assignment

Masking

ParticipantCare ProviderInvestigator

Allocation

Randomized

Enrollment

52 (Actual)

8. Arms, Groups, and Interventions

Arm Title

Losartan

Arm Type

Experimental

Arm Title

Sugar Pill

Arm Type

Placebo Comparator

Intervention Type

Drug

Intervention Name(s)

Losartan

Other Intervention Name(s)

Cozaar

Intervention Description

Participants will start with 50 mg of losartan by mouth daily. The dose will be increased to 100 mg by mouth daily after 14 days. The maximal tolerable dosage (up to 100mg by mouth daily) will be continued for a total of 30 months.

Intervention Type

Drug

Intervention Name(s)

Placebo

Intervention Description

one tablet by mouth daily

Primary Outcome Measure Information:

Title

Collagen Deposition in LT

Description

Time Frame

30 months

Title

Integrity of the Fibroblastic Reticular Cell Network (FRCn)

Description

Time Frame

30 months

Secondary Outcome Measure Information:

Title

Frequency of CD4+ T Cells

Description

Impact of losartan on immune reconstitution and function will be determined by frequency of CD4+ T cells in LT using IHC.

Time Frame

30 months

Title

Frequency TUNEL+CD3+CD8+ T Cells

Description

Impact of losartan on immune reconstitution and function will be determined by frequency of TUNEL+CD3+CD8+ T cells in LT using IHC.

Time Frame

30 months

Title

Frequency of Cells Expressing TGF-beta and Lymphotoxin-beta

Description

Impact of losartan on immune reconstitution and function will be determined by frequency of cells expressing TGF-beta and lymphotoxin-beta in LT using IHC.

Time Frame

30 months

Title

Serum Concentration of IL-7

Description

Impact of losartan on immune reconstitution and function will be determine by serum concentrations of IL-7 measured with ELISA.

Time Frame

30 months

Title

Serum Concentration of TGF-beta

Description

Impact of losartan on immune reconstitution and function will be determine by serum concentrations of TGF-beta measured with ELISA.

Time Frame

30 months

Title

Immune Response to HPV Vaccination

Description

Time Frame

30 months

Title

Frequency of Activated T-cell Populations - Immunofluorescent Staining

Description

Time Frame

30 months

Title

Percent of Activated T Cells in PBMCs - Flow Cytometry

Description

Time Frame

30 months

Title

Percent of Activated Macrophages in PBMCs - Flow Cytometry

Description

Time Frame

30 months

Title

Percent of Activated Dendritic Cells in PBMCs - Flow Cytometry

Description

Time Frame

30 months

Title

Percent of Activated T Cells in LT - Flow Cytometry

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the percentage of activated T cells in lymphoid tissues (LT) using flow cytometry.

Time Frame

30 months

Title

Percent of Activated Macrophages in LT - Flow Cytometry

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the percentage of activated macrophages in lymphoid tissues (LT) using flow cytometry.

Time Frame

30 months

Title

Percent of Activated Dendritic Cells in LT - Flow Cytometry

Description

Time Frame

30 months

Title

Intracellular Concentration of IL-17 in PBMCs

Description

Time Frame

30 months

Title

Intracellular Concentration of IFNg in PBMCs

Description

Time Frame

30 months

Title

Intracellular Concentration of IL-2 in PBMCs

Description

Time Frame

30 months

Title

Intracellular Concentration of TNF in PBMCs

Description

Time Frame

30 months

Title

Intracellular Concentration of IL-10 in PBMCs

Description

Time Frame

30 months

Title

Intracellular Concentration of GM-CSF in PBMCs

Description

Time Frame

30 months

Title

Intracellular Concentration of IL-17 in LT

Description

Time Frame

30 months

Title

Intracellular Concentration of IFNg in LT

Description

Time Frame

30 months

Title

Intracellular Concentration of IL-2 in LT

Description

Time Frame

30 months

Title

Intracellular Concentration of TNF in LT

Description

Time Frame

30 months

Title

Intracellular Concentration of IL-10 in LT

Description

Time Frame

30 months

Title

Intracellular Concentration of GM-CSF in LT

Description

Time Frame

30 months

Title

Plasma Concentration of LPS

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of LPS by ELISA.

Time Frame

30 months

Title

Plasma Concentration of sCD14

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of sCD14 by limulus assay.

Time Frame

30 months

Title

Plasma Concentration of I-FABP

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of I-FABP using ELISA.

Time Frame

30 months

Title

Plasma Concentration of IL-1b

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of IL-1b using ELISA.

Time Frame

30 months

Title

Plasma Concentration of IL-1RA

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of IL-1RA using ELISA.

Time Frame

30 months

Title

Plasma Concentration of IL-6

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of IL-6 using ELISA.

Time Frame

30 months

Title

Plasma Concentration of TNF

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of TNF using ELISA.

Time Frame

30 months

Title

Plasma Concentration of Amyloid A

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of amyloid A using ELISA.

Time Frame

30 months

Title

Plasma Concentration of CRP

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of CRP using ELISA.

Time Frame

30 months

Title

Plasma Concentration of D-dimer

Description

The Impact of Losartan on Immune Activation in HIV Infected, Treated Individuals will be determined by measuring the plasma concentration of D-dimer using ELISA.

Time Frame

30 months

Title

Frequency of HIV RNA+ and DNA+ Cells in LN - Radiolabeled ISH

Description

The Potential for Losartan to Reduce the Size of the Viral Reservoir will be assessed by determining the frequency of HIV RNA+ and DNA+ cells in LN using radiolabeled in situ hybridization (ISH).

Time Frame

30 months

Title

Frequency of HIV RNA+ and DNA+ Cells in LN - RNAscopeTM in Situ Technology

Description

The Potential for Losartan to Reduce the Size of the Viral Reservoir will be assessed by determining the frequency of HIV RNA+ and DNA+ cells in LN using RNAscopeTM in situ technology.

Time Frame

30 months

Title

Frequency of HIV RNA+ and DNA+ Cells in GALT - Radiolabeled in Situ Hybridization (ISH)

Description

The Potential for Losartan to Reduce the Size of the Viral Reservoir will be assessed by determining the frequency of HIV RNA+ and DNA+ cells in GALT radiolabeled in situ hybridization (ISH).

Time Frame

30 months

Title

Frequency of HIV RNA+ and DNA+ Cells in GALT - RNAscopeTM in Situ Technology

Description

The Potential for Losartan to Reduce the Size of the Viral Reservoir will be assessed by determining the frequency of HIV RNA+ and DNA+ cells in GALT using RNAscopeTM in situ technology.

Time Frame

30 months

Title

Concentration of Losartan and Antiretrovirals (ARVs)

Description

Potential Drug-drug Interactions Between Losartan and Antiretrovirals (ARVs) will be assessed by measuring levels of ARVs and losartan in plasma and peripheral blood mononuclear cells (PBMCs).

Time Frame

30 months

Title

Intracellular Concentration of Losartan and Antiretrovirals (ARVs)

Description

Potential Drug-drug Interactions Between Losartan and Antiretrovirals (ARVs) will be assessed by measuring intracellular concentration of losartan and ARVs in lympoidtissue.

Time Frame

30 months

Other Pre-specified Outcome Measures:

Title

Frequency of Dendritic Cell and CD4 T Cell Interactions With the FRCn

Description

As an exploratory endpoint, we will determine the impact of losartan on frequency of dendritic cell and CD4 T cell interactions with the FRCn. This will be determined using two-photon microscopy in sections on LN obtained from study subjects. Given that this is an exploratory endpoint, these assays will be performed in a subset of subjects (5 losartan treated, 2 placebo treated and 5 HIV uninfected controls).

Time Frame

30 months

10. Eligibility

Sex

All

Minimum Age & Unit of Time

18 Years

Accepts Healthy Volunteers

Eligibility Criteria

HIV infected participants: Inclusion Criteria: Participants must meet all of the following inclusion criteria to participate in this study: HIV-1 infected. -≥ 18 years of age. Baseline peripheral CD4+ T cell count 200-600 cells/mm3 for at least two measures over the 6 months prior to study enrollment. -≥ 12 months of stable ART, defined as use of a given drug regimen without disruption lasting ≥ 1 week in the period leading up to study enrollment. HIV viral load (VL) < 50 copies/mL for at least two consecutive measures over the 6 months prior to study enrollment. No contraindication to proposed study procedures. Women of child-bearing potential must be willing to use a form of effective contraception for the duration of the study. Effective contraception includes hormonal injection, implant or oral medication, IUD, diaphragm, or cervical cap with spermicide. Condoms cannot be used as the sole form of contraception. Exclusion Criteria: Participants meeting any of the following exclusion criteria at baseline will be excluded from study participation: Use of any immunomodulator within the 12 months prior to study enrollment. An immunomodulator for the purposes of this study is defined as a drug known to either diminish or augment a patient's immune system. Examples of these include, but are not limited to, systemic corticosteroids (use of topical steroids will be permitted), TNF-inhibitors, rituximab, cyclophosphamide, abatacept,cyclosporine, azathioprine, 6-mercaptopurine, methotrexate, sulfasalazine, cyclosporine, tacrolimus,sirolimus, and intravenous immune globulin. Current use of an ARB or ACEi. Current use of rifaximin, fluconazole or lithium given potential for drug interactions with losartan. Prior reaction or intolerance to an ARB or ACEi. Prior diagnosis of a chronic inflammatory disease with serologic or clinical evidence as diagnosed by a primary care physician or specialist. Examples of these include, but are not limited to, systemic lupus erythematosus, rheumatoid arthritis, scleroderma, Sjogren's syndrome, mixed connective tissue disease, psoriasis, polymyositis, dermatomyositis, vasculitis, sarcoidosis, Wegener's granulomatosis, giant cell arteritis, polyarteritis nodosa, gastrointestinal pemphigoid, eosinophilic colitis, Crohn's disease, ulcerative colitis, autoimmune hepatitis, and hepatitis C. Prior diagnosis of a connective tissue disease with genetic, serologic or clinical evidence as diagnosed by a primary care physician or specialist (Marfan's syndrome, Ehlers-Danlos syndrome). Baseline blood pressure < 110/70. Estimated Glomerular Filtration Rate (eGFR) of < 30ml/min/1.73 m2 within 4 weeks of study initiation or history of advanced renal disease. AST and/or ALT > 3 times the upper limit of normal within 4 weeks of study enrollment. Potassium > 5.0 within 4 weeks of study enrollment. Pregnancy. In women of childbearing age, unwillingness to use birth control for the duration of the study. Breast feeding. Prior vaccination with an HPV vaccine, including Cervarix (GlaxoSmithKline) or Gardasil (Merck). History of hypersensitivity or severe allergic reactions to yeast. HIV-uninfected: Inclusion Criteria Participants must meet all of the following inclusion criteria to participate in this study: HIV uninfected. -≥ 18 years of age. No contraindication to proposed study procedures. Exclusion Criteria: Participants meeting any of the following exclusion criteria at baseline will be excluded from study participation: Use of any immunomodulator within the 12 months prior to study enrollment (as defined above). Current use of an ARB or ACEi. Prior diagnosis of a chronic inflammatory disease with serologic or clinical evidence (as defined above). Prior diagnosis of a connective tissue disease with genetic, serologic or clinical evidence as diagnosed by a primary care physician or specialist (Marfan's syndrome, Ehlers-Danlos syndrome). Pregnancy.

Overall Study Officials:

First Name & Middle Initial & Last Name & Degree

Timothy Schacker, M.D.

Organizational Affiliation

University of Minnesota

Official's Role

Principal Investigator

Facility Information:

Facility Name

University of Minnesota, Division of Infectious Diseases

City

Minneapolis

State/Province

Minnesota

ZIP/Postal Code

55455

Country

United States

12. IPD Sharing Statement

Learn more about this trial

Reversing Tissue Fibrosis to Improve Immune Reconstitution in HIV

We'll reach out to this number within 24 hrs