Alveolar macrophage apoptosis-associated bacterial killing helps prevent murine pneumonia

Julie A Preston; Martin A Bewley; Helen M Marriott; A McGarry Houghton; Mohamed Mohasin; Jamil Jubrail; Lucy Morris; Yvonne L Stephenson; Simon Cross; David R Greaves; Ruth W Craig; Nico van Rooijen; Colin D Bingle; Robert C Read; Timothy J Mitchell; Moira K B Whyte; Steven D Shapiro; David H Dockrell

doi:10.1164/rccm.201804-0646OC

Alveolar macrophage apoptosis-associated bacterial killing helps prevent murine pneumonia

Julie A Preston, Martin A Bewley, Helen M Marriott, A McGarry Houghton, Mohamed Mohasin, Jamil Jubrail, Lucy Morris, Yvonne L Stephenson, Simon Cross, David R Greaves, Ruth W Craig, Nico van Rooijen, Colin D Bingle, Robert C Read, Timothy J Mitchell, Moira K B Whyte, Steven D Shapiro, David H Dockrell

Microbiology and Infection

Research output: Contribution to journal › Article › peer-review

15 Citations (Scopus)

Abstract

Rationale: Antimicrobial resistance challenges therapy of pneumonia. Enhancing macrophage microbicidal responses would combat this problem but is limited by our understanding of how alveolar macrophages (AMs) kill bacteria. Objectives: To define the role and mechanism of AM apoptosis-associated bacterial killing in the lung. Methods: We generated a unique CD68.hMcl-1 transgenic mouse with macrophage-specific overexpression of the human antiapoptotic Mcl-1 protein, a factor upregulated in AMs from patients at increased risk of community-acquired pneumonia, to address the requirement for apoptosis-associated killing. Measurements and Main Results: Wild-type and transgenic macrophages demonstrated comparable ingestion and initial phagolysosomal killing of bacteria. Continued ingestion (for >12 h) overwhelmed initial killing, and a second, late-phase microbicidal response killed viable bacteria in wild-type macrophages, but this response was blunted in CD68.hMcl-1 transgenic macrophages. The late phase of bacterial killing required both caspase-induced generation of mitochondrial reactive oxygen species and nitric oxide, the peak generation of which coincided with the late phase of killing. The CD68.hMcl-1 transgene prevented mitochondrial reactive oxygen species but not nitric oxide generation. Apoptosis-associated killing enhanced pulmonary clearance of Streptococcus pneumoniae and Haemophilus influenzae in wild-type mice but not CD68.hMcl-1 transgenic mice. Bacterial clearance was enhanced in vivo in CD68.hMcl-1 transgenic mice by reconstitution of apoptosis with BH3 mimetics or clodronate-encapsulated liposomes. Apoptosis-associated killing was not activated during Staphylococcus aureus lung infection. Conclusions: Mcl-1 upregulation prevents macrophage apoptosis-associated killing and establishes that apoptosis-associated killing is required to allow AMs to clear ingested bacteria. Engagement of macrophage apoptosis should be investigated as a novel, host-based antimicrobial strategy.

Original language	English
Pages (from-to)	84-97
Number of pages	14
Journal	American Journal of Respiratory and Critical Care Medicine
Volume	200
Issue number	1
Early online date	16 Jan 2019
DOIs	https://doi.org/10.1164/rccm.201804-0646OC
Publication status	Published - 1 Jul 2019

Keywords

Apoptosis
Bacteria
Macrophage
Mcl-1
Pneumonia

Access to Document

10.1164/rccm.201804-0646OCLicence: None: All rights reserved

http://eprints.whiterose.ac.uk/141496/Licence: None: All rights reserved

Cite this

Preston, J. A., Bewley, M. A., Marriott, H. M., Houghton, A. M., Mohasin, M., Jubrail, J., Morris, L., Stephenson, Y. L., Cross, S., Greaves, D. R., Craig, R. W., van Rooijen, N., Bingle, C. D., Read, R. C., Mitchell, T. J., Whyte, M. K. B., Shapiro, S. D., & Dockrell, D. H. (2019). Alveolar macrophage apoptosis-associated bacterial killing helps prevent murine pneumonia. American Journal of Respiratory and Critical Care Medicine, 200(1), 84-97. Advance online publication. https://doi.org/10.1164/rccm.201804-0646OC

@article{22ce079512be43fbb5f2b49ebc635251,

title = "Alveolar macrophage apoptosis-associated bacterial killing helps prevent murine pneumonia",

abstract = "Rationale: Antimicrobial resistance challenges therapy of pneumonia. Enhancing macrophage microbicidal responses would combat this problem but is limited by our understanding of how alveolar macrophages (AMs) kill bacteria. Objectives: To define the role and mechanism of AM apoptosis-associated bacterial killing in the lung. Methods: We generated a unique CD68.hMcl-1 transgenic mouse with macrophage-specific overexpression of the human antiapoptotic Mcl-1 protein, a factor upregulated in AMs from patients at increased risk of community-acquired pneumonia, to address the requirement for apoptosis-associated killing. Measurements and Main Results: Wild-type and transgenic macrophages demonstrated comparable ingestion and initial phagolysosomal killing of bacteria. Continued ingestion (for >12 h) overwhelmed initial killing, and a second, late-phase microbicidal response killed viable bacteria in wild-type macrophages, but this response was blunted in CD68.hMcl-1 transgenic macrophages. The late phase of bacterial killing required both caspase-induced generation of mitochondrial reactive oxygen species and nitric oxide, the peak generation of which coincided with the late phase of killing. The CD68.hMcl-1 transgene prevented mitochondrial reactive oxygen species but not nitric oxide generation. Apoptosis-associated killing enhanced pulmonary clearance of Streptococcus pneumoniae and Haemophilus influenzae in wild-type mice but not CD68.hMcl-1 transgenic mice. Bacterial clearance was enhanced in vivo in CD68.hMcl-1 transgenic mice by reconstitution of apoptosis with BH3 mimetics or clodronate-encapsulated liposomes. Apoptosis-associated killing was not activated during Staphylococcus aureus lung infection. Conclusions: Mcl-1 upregulation prevents macrophage apoptosis-associated killing and establishes that apoptosis-associated killing is required to allow AMs to clear ingested bacteria. Engagement of macrophage apoptosis should be investigated as a novel, host-based antimicrobial strategy.",

keywords = "Apoptosis, Bacteria, Macrophage, Mcl-1, Pneumonia",

author = "Preston, {Julie A} and Bewley, {Martin A} and Marriott, {Helen M} and Houghton, {A McGarry} and Mohamed Mohasin and Jamil Jubrail and Lucy Morris and Stephenson, {Yvonne L} and Simon Cross and Greaves, {David R} and Craig, {Ruth W} and {van Rooijen}, Nico and Bingle, {Colin D} and Read, {Robert C} and Mitchell, {Timothy J} and Whyte, {Moira K B} and Shapiro, {Steven D} and Dockrell, {David H}",

year = "2019",

month = jul,

day = "1",

doi = "10.1164/rccm.201804-0646OC",

language = "English",

volume = "200",

pages = "84--97",

journal = "American Journal of Respiratory and Critical Care Medicine",

issn = "1073-449X",

publisher = "American Thoracic Society",

number = "1",

}

Preston, JA, Bewley, MA, Marriott, HM, Houghton, AM, Mohasin, M, Jubrail, J, Morris, L, Stephenson, YL, Cross, S, Greaves, DR, Craig, RW, van Rooijen, N, Bingle, CD, Read, RC, Mitchell, TJ, Whyte, MKB, Shapiro, SD & Dockrell, DH 2019, 'Alveolar macrophage apoptosis-associated bacterial killing helps prevent murine pneumonia', American Journal of Respiratory and Critical Care Medicine, vol. 200, no. 1, pp. 84-97. https://doi.org/10.1164/rccm.201804-0646OC

TY - JOUR

T1 - Alveolar macrophage apoptosis-associated bacterial killing helps prevent murine pneumonia

AU - Preston, Julie A

AU - Bewley, Martin A

AU - Marriott, Helen M

AU - Houghton, A McGarry

AU - Mohasin, Mohamed

AU - Jubrail, Jamil

AU - Morris, Lucy

AU - Stephenson, Yvonne L

AU - Cross, Simon

AU - Greaves, David R

AU - Craig, Ruth W

AU - van Rooijen, Nico

AU - Bingle, Colin D

AU - Read, Robert C

AU - Mitchell, Timothy J

AU - Whyte, Moira K B

AU - Shapiro, Steven D

AU - Dockrell, David H

PY - 2019/7/1

Y1 - 2019/7/1

N2 - Rationale: Antimicrobial resistance challenges therapy of pneumonia. Enhancing macrophage microbicidal responses would combat this problem but is limited by our understanding of how alveolar macrophages (AMs) kill bacteria. Objectives: To define the role and mechanism of AM apoptosis-associated bacterial killing in the lung. Methods: We generated a unique CD68.hMcl-1 transgenic mouse with macrophage-specific overexpression of the human antiapoptotic Mcl-1 protein, a factor upregulated in AMs from patients at increased risk of community-acquired pneumonia, to address the requirement for apoptosis-associated killing. Measurements and Main Results: Wild-type and transgenic macrophages demonstrated comparable ingestion and initial phagolysosomal killing of bacteria. Continued ingestion (for >12 h) overwhelmed initial killing, and a second, late-phase microbicidal response killed viable bacteria in wild-type macrophages, but this response was blunted in CD68.hMcl-1 transgenic macrophages. The late phase of bacterial killing required both caspase-induced generation of mitochondrial reactive oxygen species and nitric oxide, the peak generation of which coincided with the late phase of killing. The CD68.hMcl-1 transgene prevented mitochondrial reactive oxygen species but not nitric oxide generation. Apoptosis-associated killing enhanced pulmonary clearance of Streptococcus pneumoniae and Haemophilus influenzae in wild-type mice but not CD68.hMcl-1 transgenic mice. Bacterial clearance was enhanced in vivo in CD68.hMcl-1 transgenic mice by reconstitution of apoptosis with BH3 mimetics or clodronate-encapsulated liposomes. Apoptosis-associated killing was not activated during Staphylococcus aureus lung infection. Conclusions: Mcl-1 upregulation prevents macrophage apoptosis-associated killing and establishes that apoptosis-associated killing is required to allow AMs to clear ingested bacteria. Engagement of macrophage apoptosis should be investigated as a novel, host-based antimicrobial strategy.

AB - Rationale: Antimicrobial resistance challenges therapy of pneumonia. Enhancing macrophage microbicidal responses would combat this problem but is limited by our understanding of how alveolar macrophages (AMs) kill bacteria. Objectives: To define the role and mechanism of AM apoptosis-associated bacterial killing in the lung. Methods: We generated a unique CD68.hMcl-1 transgenic mouse with macrophage-specific overexpression of the human antiapoptotic Mcl-1 protein, a factor upregulated in AMs from patients at increased risk of community-acquired pneumonia, to address the requirement for apoptosis-associated killing. Measurements and Main Results: Wild-type and transgenic macrophages demonstrated comparable ingestion and initial phagolysosomal killing of bacteria. Continued ingestion (for >12 h) overwhelmed initial killing, and a second, late-phase microbicidal response killed viable bacteria in wild-type macrophages, but this response was blunted in CD68.hMcl-1 transgenic macrophages. The late phase of bacterial killing required both caspase-induced generation of mitochondrial reactive oxygen species and nitric oxide, the peak generation of which coincided with the late phase of killing. The CD68.hMcl-1 transgene prevented mitochondrial reactive oxygen species but not nitric oxide generation. Apoptosis-associated killing enhanced pulmonary clearance of Streptococcus pneumoniae and Haemophilus influenzae in wild-type mice but not CD68.hMcl-1 transgenic mice. Bacterial clearance was enhanced in vivo in CD68.hMcl-1 transgenic mice by reconstitution of apoptosis with BH3 mimetics or clodronate-encapsulated liposomes. Apoptosis-associated killing was not activated during Staphylococcus aureus lung infection. Conclusions: Mcl-1 upregulation prevents macrophage apoptosis-associated killing and establishes that apoptosis-associated killing is required to allow AMs to clear ingested bacteria. Engagement of macrophage apoptosis should be investigated as a novel, host-based antimicrobial strategy.

KW - Apoptosis

KW - Bacteria

KW - Macrophage

KW - Mcl-1

KW - Pneumonia

UR - http://www.scopus.com/inward/record.url?scp=85068411045&partnerID=8YFLogxK

U2 - 10.1164/rccm.201804-0646OC

DO - 10.1164/rccm.201804-0646OC

M3 - Article

C2 - 30649895

SN - 1073-449X

VL - 200

SP - 84

EP - 97

JO - American Journal of Respiratory and Critical Care Medicine

JF - American Journal of Respiratory and Critical Care Medicine

IS - 1

ER -

Alveolar macrophage apoptosis-associated bacterial killing helps prevent murine pneumonia

Abstract

Keywords

Access to Document

Fingerprint

Cite this