Nicotine at physiologic concentrations impairs macrophage killing of Mycobacterium tuberculosis (MTB), resulting in a 2-5 fold increase in bacterial burden. We have also found that preventing nicotine binding ? either pharmacologically or by genetic disruption of the nicotinic receptor ? significantly mitigated cigarette smoke extract-induced impairment of macrophage killing of MTB. But the mechanisms by which nicotine impairs macrophage control of MTB are not known. Our hypothesis is that nicotine sabotages macrophage function against MTB (i) directly through NF?B-mediated inhibition of autophagy and apoptosis as well as through DICER/microRNA-mediated inhibition of host-protective cytokine production and (ii) indirectly through increased production of CTLA-4 and activation of T regulatory cells (Tregs).
Aim 1 : Determine the mechanisms by which nicotine directly impairs macrophage killing of MTB. Approach: We will isolate nicotine-nave human alveolar macrophages (AM) and monocyte-derived macrophages (MDM), infect them with MTB nicotine, and quantify autophagy, apoptosis, intracellular burden of MTB, and the extent NF?B inhibition mitigates the effects of nicotine. We will also knockdown specific NF?B subunits and DICER to determine their roles in nicotine-mediated inhibition of anti-MTB immunity. Hypothesis: Nicotine induction of NF?B in AM and MDM will inhibit autophagy and apoptosis, resulting in increased burden of MTB. Inhibition of NF?B activation will abrogate these effects of nicotine and restore macrophage killing of MTB. Knockdown of DICER will reverse the suppression of MTB-induced cytokines by nicotine.
Aim 2 : Determine the mechanisms by which nicotine indirectly impairs macrophage killing of MTB.
Sub aim A. An ex vivo model using primary human cells. Approach: We will culture nave human MDM with nave vs. nicotine-exposed Tregs and infect the cells with MTB. To determine if CTLA-4 expression is responsible for nicotine-induced increase in Treg activity and secondary MDM suppression, the cells will also be incubated with anti-CTLA-4 neutralizing antibody. Hypothesis: Nicotine will increase CTLA-4 expression on Tregs, augmenting their production of IL-10 and TGF?. This will inhibit autophagy in MTB-infected MDM and result in greater bacterial burden compared to MDM co-cultured with nicotine-nave Tregs. Antagonism of CTLA-4 will abrogate these immunosuppressive effects of nicotine.
Sub aim B. In vivo murine model. Approach: We will adoptively transfer Tregs from unexposed or nicotine- exposed B6.PL(Thy1.1) mice into Treg-depleted Foxp3+GFP+DTR+(Thy1.2) mice, infect the recipient mice with MTB, and quantify MTB burden, macrophage and T cell phenotypes, lung histopathology, and survival. Hypothesis: Mice receiving nicotine-exposed Tregs will have fewer host-protective M1 lung macrophages and TH1 and TH17 cells compared to mice receiving nicotine-nave Tregs. As a result, mice receiving nicotine- exposed Tregs will be more susceptible to MTB, demonstrated by greater MTB burden, fewer host-protective macrophages and T helper phenotypes, more severe lung pathology, and decreased survival. Potential impact of project: U.S. Veterans have a high prevalence of nicotine exposure (through use of cigarette smoke and smokeless nicotine products) and a greater risk for TB due to overseas deployment in TB endemic countries, relatively high prevalence of homelessness, and advancing age. While nicotine impairs human macrophage control of MTB, no work has been conducted to determine how this occurs; illuminating these mechanisms will provide the scientific impetus to help alert the medical and public health communities of this danger of concomitant nicotine and MTB exposures in veterans and non-veterans. Findings from these studies can also provide the foundation for developing immunomodulatory approaches to treatment even in the absence of nicotine exposure; e.g., use of clinically available anti-CTLA-4 agents to deactivate Tregs in an attempt to optimize host immunity against TB.

Public Health Relevance

The increased risk for tuberculosis (TB) with nicotine exposure is of concern to veteran health because veterans have: (i) a relatively high rate of nicotine exposure and (ii) higher rate of acquiring TB due to deployment in TB-endemic countries, relatively high prevalence of homelessness, and the aging veteran population. Nicotine impairs macrophage killing of Mycobacterium tuberculosis (MTB) but the mechanisms are not known. The goal of this project is to uncover the mechanisms using both primary human lung and blood cells and a mouse model. Pharmacologic agents with the potential to enhance host immunity will also be tested to determine if they can negate the effects of nicotine.

Agency
National Institute of Health (NIH)
Institute
Veterans Affairs (VA)
Type
Non-HHS Research Projects (I01)
Project #
1I01CX001452-01A1
Application #
9241192
Study Section
Infectious Diseases B (INFB)
Project Start
2017-10-01
Project End
2021-09-30
Budget Start
2017-10-01
Budget End
2018-09-30
Support Year
1
Fiscal Year
2018
Total Cost
Indirect Cost
Name
VA Eastern Colorado Health Care System
Department
Type
DUNS #
003252830
City
Aurora
State
CO
Country
United States
Zip Code
80045
Bai, Xiyuan; Aerts, Shanae L; Verma, Deepshikha et al. (2018) Epidemiologic Evidence of and Potential Mechanisms by Which Second-Hand Smoke Causes Predisposition to Latent and Active Tuberculosis. Immune Netw 18:e22
Bai, Xiyuan; Stitzel, Jerry A; Bai, An et al. (2017) Nicotine Impairs Macrophage Control of Mycobacterium tuberculosis. Am J Respir Cell Mol Biol 57:324-333