Magnetic-activated cell sorting identifies a unique lung microbiome community

Daniel G Dunlap; Libing Yang; Shulin Qin; Kelvin Li; Adam Fitch; Laurence Huang; Bryan J McVerry; Timothy W Hand; Barbara A Methé; Alison Morris

doi:10.1186/s40168-022-01434-5

Magnetic-activated cell sorting identifies a unique lung microbiome community

Microbiome. 2023 May 25;11(1):117. doi: 10.1186/s40168-022-01434-5.

Authors

Daniel G Dunlap^{1

2}, Libing Yang^{3

4}, Shulin Qin^{3

4}, Kelvin Li⁴, Adam Fitch⁴, Laurence Huang⁵, Bryan J McVerry³, Timothy W Hand⁶, Barbara A Methé⁴, Alison Morris^{3

4

7}

Affiliations

¹ Division of Pulmonary, Allergy and Critical Care Medicine, Department of Medicine, University of Pittsburgh School of Medicine and University of Pittsburgh Medical Center, NW628, 3459 Fifth Avenue, Pittsburgh, PA, 15213, USA. dunlapd2@upmc.edu.
² Center for Medicine and the Microbiome, University of Pittsburgh, Pittsburgh, USA. dunlapd2@upmc.edu.
³ Division of Pulmonary, Allergy and Critical Care Medicine, Department of Medicine, University of Pittsburgh School of Medicine and University of Pittsburgh Medical Center, NW628, 3459 Fifth Avenue, Pittsburgh, PA, 15213, USA.
⁴ Center for Medicine and the Microbiome, University of Pittsburgh, Pittsburgh, USA.
⁵ Department of Medicine, University of California, San Francisco, CA, USA.
⁶ Children's Hospital of Pittsburgh, Pittsburgh, PA, USA.
⁷ Department of Immunology, University of Pittsburgh School of Medicine, Pittsburgh, PA, USA.

Abstract

Background: The advent of culture-independent, next-generation DNA sequencing has led to the discovery of distinct lung bacterial communities. Studies of lung microbiome taxonomy often reveal only subtle differences between health and disease, but host recognition and response may distinguish the members of similar bacterial communities in different populations. Magnetic-activated cell sorting has been applied to the gut microbiome to identify the numbers and types of bacteria eliciting a humoral response. We adapted this technique to examine the populations of immunoglobulin-bound bacteria in the lung.

Methods: Sixty-four individuals underwent bronchoalveolar lavage (BAL). We separated immunoglobulin G-bound bacteria using magnetic-activated cell sorting and sequenced the 16S rRNA gene on the Illumina MiSeq platform. We compared microbial sequencing data in IgG-bound bacterial communities compared to raw BAL then examined the differences in individuals with and without HIV as a representative disease state.

Results: Immunoglobulin G-bound bacteria were identified in all individuals. The community structure differed when compared to raw BAL, and there was a greater abundance of Pseudomonas and fewer oral bacteria in IgG-bound BAL. Examination of IgG-bound communities in individuals with HIV demonstrated the differences in Ig-bound bacteria by HIV status that were not seen in a comparison of raw BAL, and greater numbers of immunoglobulin-bound bacteria were associated with higher pulmonary cytokine levels.

Conclusions: We report a novel application of magnetic-activated cell sorting to identify immunoglobulin G-bound bacteria in the lung. This technique identified distinct bacterial communities which differed in composition from raw bronchoalveolar lavage, revealing the differences not detected by traditional analyses. Cytokine response was also associated with differential immunoglobulin binding of lung bacteria, suggesting the functional importance of these communities. Video Abstract.

Keywords: Host response; Immunoglobulin; Microbiome.

Publication types

Video-Audio Media
Research Support, N.I.H., Extramural

MeSH terms

Cytokines
Dimercaprol
HIV Infections*
Humans
Immunoglobulin G
Magnetic Phenomena
Microbiota* / genetics
RNA, Ribosomal, 16S / genetics

Substances

RNA, Ribosomal, 16S
Immunoglobulin G
Cytokines
Dimercaprol

Abstract

Publication types

MeSH terms

Substances

Grants and funding