Enhancing responsiveness of human jejunal enteroids to host and microbial stimuli

Wenly Ruan; Melinda A. Engevik; Alexandra L. Chang-Graham; Heather A. Danhof; Annie Goodwin; Kristen A. Engevik; Zhongcheng Shi; Anne Hall; Sara C.Di Rienzi; Susan Venable; Robert A. Britton; Joseph Hyser; James Versalovic

doi:10.1113/JP279423

Enhancing responsiveness of human jejunal enteroids to host and microbial stimuli

Wenly Ruan, Melinda A. Engevik, Alexandra L. Chang-Graham, Heather A. Danhof, Annie Goodwin, Kristen A. Engevik, Zhongcheng Shi, Anne Hall, Sara C.Di Rienzi, Susan Venable, Robert A. Britton, Joseph Hyser, James Versalovic

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

15 Scopus citations

Abstract

Key points: Enteroids are a physiologically relevant model to examine the human intestine and its functions. Previously, the measurable cytokine response of human intestinal enteroids has been limited following exposure to host or microbial pro-inflammatory stimuli. Modifications to enteroid culture conditions facilitated robust human cytokine responses to pro-inflammatory stimuli. This new human enteroid culture methodology refines the ability to study microbiome:human intestinal epithelium interactions in the laboratory. Abstract: The intestinal epithelium is the primary interface between the host, the gut microbiome and its external environment. Since the intestinal epithelium contributes to innate immunity as a first line of defence, understanding how the epithelium responds to microbial and host stimuli is an important consideration in promoting homeostasis. Human intestinal enteroids (HIEs) are primary epithelial cell cultures that can provide insights into the biology of the intestinal epithelium and innate immune responses. One potential limitation of using HIEs for innate immune studies is the relative lack of responsiveness to factors that stimulate epithelial cytokine production. We report technical refinements, including removal of extracellular antioxidants, to facilitate enhanced cytokine responses in HIEs. Using this new method, we demonstrate that HIEs have distinct cytokine profiles in response to pro-inflammatory stimuli derived from host and microbial sources. Overall, we found that host-derived cytokines tumour necrosis factor and interleukin-1α stimulated reactive oxygen species and a large repertoire of cytokines. In contrast, microbial lipopolysaccharide, lipoteichoic acid and flagellin stimulated a limited number of cytokines and histamine did not stimulate the release of any cytokines. Importantly, HIE-secreted cytokines were functionally active, as denoted by the ability of human blood-derived neutrophil to migrate towards HIE supernatant containing interleukin-8. These findings establish that the immune responsiveness of HIEs depends on medium composition and stimuli. By refining the experimental culture medium and creating an environment conducive to epithelial cytokine responses by human enteroids, HIEs can facilitate exploration of many experimental questions pertaining to the role of the intestinal epithelium in innate immunity.

Original language	English (US)
Pages (from-to)	3085-3105
Number of pages	21
Journal	Journal of Physiology
Volume	598
Issue number	15
DOIs	https://doi.org/10.1113/JP279423
State	Published - Aug 1 2020

Keywords

cytokine
flagellin
histamine
human intestinal enteroids (HIEs)
toll-like receptors (TLR)
tumor necrosis factor (TNF)
Intestinal Mucosa
Intestines
Jejunum
Humans
Epithelial Cells
Immunity, Innate

ASJC Scopus subject areas

Physiology

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10.1113/JP279423

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@article{74b739acba534b82a04ee42e1b80b493,

title = "Enhancing responsiveness of human jejunal enteroids to host and microbial stimuli",

abstract = "Key points: Enteroids are a physiologically relevant model to examine the human intestine and its functions. Previously, the measurable cytokine response of human intestinal enteroids has been limited following exposure to host or microbial pro-inflammatory stimuli. Modifications to enteroid culture conditions facilitated robust human cytokine responses to pro-inflammatory stimuli. This new human enteroid culture methodology refines the ability to study microbiome:human intestinal epithelium interactions in the laboratory. Abstract: The intestinal epithelium is the primary interface between the host, the gut microbiome and its external environment. Since the intestinal epithelium contributes to innate immunity as a first line of defence, understanding how the epithelium responds to microbial and host stimuli is an important consideration in promoting homeostasis. Human intestinal enteroids (HIEs) are primary epithelial cell cultures that can provide insights into the biology of the intestinal epithelium and innate immune responses. One potential limitation of using HIEs for innate immune studies is the relative lack of responsiveness to factors that stimulate epithelial cytokine production. We report technical refinements, including removal of extracellular antioxidants, to facilitate enhanced cytokine responses in HIEs. Using this new method, we demonstrate that HIEs have distinct cytokine profiles in response to pro-inflammatory stimuli derived from host and microbial sources. Overall, we found that host-derived cytokines tumour necrosis factor and interleukin-1α stimulated reactive oxygen species and a large repertoire of cytokines. In contrast, microbial lipopolysaccharide, lipoteichoic acid and flagellin stimulated a limited number of cytokines and histamine did not stimulate the release of any cytokines. Importantly, HIE-secreted cytokines were functionally active, as denoted by the ability of human blood-derived neutrophil to migrate towards HIE supernatant containing interleukin-8. These findings establish that the immune responsiveness of HIEs depends on medium composition and stimuli. By refining the experimental culture medium and creating an environment conducive to epithelial cytokine responses by human enteroids, HIEs can facilitate exploration of many experimental questions pertaining to the role of the intestinal epithelium in innate immunity.",

keywords = "cytokine, flagellin, histamine, human intestinal enteroids (HIEs), toll-like receptors (TLR), tumor necrosis factor (TNF), Intestinal Mucosa, Intestines, Jejunum, Humans, Epithelial Cells, Immunity, Innate",

author = "Wenly Ruan and Engevik, {Melinda A.} and Chang-Graham, {Alexandra L.} and Danhof, {Heather A.} and Annie Goodwin and Engevik, {Kristen A.} and Zhongcheng Shi and Anne Hall and Rienzi, {Sara C.Di} and Susan Venable and Britton, {Robert A.} and Joseph Hyser and James Versalovic",

note = "Funding Information: JV and RAB receive unrestricted research support from BioGaia AB, a Swedish probiotics company. JV serves on the scientific advisory board of Seed, a USA‐based probiotics/prebiotics company. JV also serves on the scientific advisory board of Biomica, an Israeli informatics enterprise and on the scientific advisory board of Plexus Worldwide, a USA‐based nutrition company. R.A. Britton serves on the scientific advisory board of Tenza, is a co‐founder of Mikrovia, and consults for Takeda and Probiotech. The remaining authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest. Funding Information: This study was supported by the NIH T32 grant 5T32DK007664-28 awarded to WR, AG and KAE. Trainee support was provided by NIH grant F30DK112563 (ACG), BCM Medical Scientist Training Program (ACG), NIH grant F32AI136404 (HAD), NLM Training Program in Biomedical Informatics and Data Science T15LM007093 (SCD), NIH P30-DK-56338 (MAE). Experiments were also made possible through the NIH U01CA170930 grant (JV), the NLM Training Program in Biomedical Informatics and Data Science T15LM007093 (SCD), and the Digestive Diseases Centre which is funded by NIH/NIDDK P30 DK56338-06A2. Funding Information: This study was supported by the NIH T32 grant 5T32DK007664‐28 awarded to WR, AG and KAE. Trainee support was provided by NIH grant F30DK112563 (ACG), BCM Medical Scientist Training Program (ACG), NIH grant F32AI136404 (HAD), NLM Training Program in Biomedical Informatics and Data Science T15LM007093 (SCD), NIH P30‐DK‐56338 (MAE). Experiments were also made possible through the NIH U01CA170930 grant (JV), the NLM Training Program in Biomedical Informatics and Data Science T15LM007093 (SCD), and the Digestive Diseases Centre which is funded by NIH/NIDDK P30 DK56338‐06A2. Publisher Copyright: {\textcopyright} 2020 The Authors. The Journal of Physiology {\textcopyright} 2020 The Physiological Society",

year = "2020",

month = aug,

day = "1",

doi = "10.1113/JP279423",

language = "English (US)",

volume = "598",

pages = "3085--3105",

journal = "Journal of Physiology",

issn = "0022-3751",

publisher = "Wiley",

number = "15",

}

TY - JOUR

T1 - Enhancing responsiveness of human jejunal enteroids to host and microbial stimuli

AU - Ruan, Wenly

AU - Engevik, Melinda A.

AU - Chang-Graham, Alexandra L.

AU - Danhof, Heather A.

AU - Goodwin, Annie

AU - Engevik, Kristen A.

AU - Shi, Zhongcheng

AU - Hall, Anne

AU - Rienzi, Sara C.Di

AU - Venable, Susan

AU - Britton, Robert A.

AU - Hyser, Joseph

AU - Versalovic, James

N1 - Funding Information: JV and RAB receive unrestricted research support from BioGaia AB, a Swedish probiotics company. JV serves on the scientific advisory board of Seed, a USA‐based probiotics/prebiotics company. JV also serves on the scientific advisory board of Biomica, an Israeli informatics enterprise and on the scientific advisory board of Plexus Worldwide, a USA‐based nutrition company. R.A. Britton serves on the scientific advisory board of Tenza, is a co‐founder of Mikrovia, and consults for Takeda and Probiotech. The remaining authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest. Funding Information: This study was supported by the NIH T32 grant 5T32DK007664-28 awarded to WR, AG and KAE. Trainee support was provided by NIH grant F30DK112563 (ACG), BCM Medical Scientist Training Program (ACG), NIH grant F32AI136404 (HAD), NLM Training Program in Biomedical Informatics and Data Science T15LM007093 (SCD), NIH P30-DK-56338 (MAE). Experiments were also made possible through the NIH U01CA170930 grant (JV), the NLM Training Program in Biomedical Informatics and Data Science T15LM007093 (SCD), and the Digestive Diseases Centre which is funded by NIH/NIDDK P30 DK56338-06A2. Funding Information: This study was supported by the NIH T32 grant 5T32DK007664‐28 awarded to WR, AG and KAE. Trainee support was provided by NIH grant F30DK112563 (ACG), BCM Medical Scientist Training Program (ACG), NIH grant F32AI136404 (HAD), NLM Training Program in Biomedical Informatics and Data Science T15LM007093 (SCD), NIH P30‐DK‐56338 (MAE). Experiments were also made possible through the NIH U01CA170930 grant (JV), the NLM Training Program in Biomedical Informatics and Data Science T15LM007093 (SCD), and the Digestive Diseases Centre which is funded by NIH/NIDDK P30 DK56338‐06A2. Publisher Copyright: © 2020 The Authors. The Journal of Physiology © 2020 The Physiological Society

PY - 2020/8/1

Y1 - 2020/8/1

N2 - Key points: Enteroids are a physiologically relevant model to examine the human intestine and its functions. Previously, the measurable cytokine response of human intestinal enteroids has been limited following exposure to host or microbial pro-inflammatory stimuli. Modifications to enteroid culture conditions facilitated robust human cytokine responses to pro-inflammatory stimuli. This new human enteroid culture methodology refines the ability to study microbiome:human intestinal epithelium interactions in the laboratory. Abstract: The intestinal epithelium is the primary interface between the host, the gut microbiome and its external environment. Since the intestinal epithelium contributes to innate immunity as a first line of defence, understanding how the epithelium responds to microbial and host stimuli is an important consideration in promoting homeostasis. Human intestinal enteroids (HIEs) are primary epithelial cell cultures that can provide insights into the biology of the intestinal epithelium and innate immune responses. One potential limitation of using HIEs for innate immune studies is the relative lack of responsiveness to factors that stimulate epithelial cytokine production. We report technical refinements, including removal of extracellular antioxidants, to facilitate enhanced cytokine responses in HIEs. Using this new method, we demonstrate that HIEs have distinct cytokine profiles in response to pro-inflammatory stimuli derived from host and microbial sources. Overall, we found that host-derived cytokines tumour necrosis factor and interleukin-1α stimulated reactive oxygen species and a large repertoire of cytokines. In contrast, microbial lipopolysaccharide, lipoteichoic acid and flagellin stimulated a limited number of cytokines and histamine did not stimulate the release of any cytokines. Importantly, HIE-secreted cytokines were functionally active, as denoted by the ability of human blood-derived neutrophil to migrate towards HIE supernatant containing interleukin-8. These findings establish that the immune responsiveness of HIEs depends on medium composition and stimuli. By refining the experimental culture medium and creating an environment conducive to epithelial cytokine responses by human enteroids, HIEs can facilitate exploration of many experimental questions pertaining to the role of the intestinal epithelium in innate immunity.

AB - Key points: Enteroids are a physiologically relevant model to examine the human intestine and its functions. Previously, the measurable cytokine response of human intestinal enteroids has been limited following exposure to host or microbial pro-inflammatory stimuli. Modifications to enteroid culture conditions facilitated robust human cytokine responses to pro-inflammatory stimuli. This new human enteroid culture methodology refines the ability to study microbiome:human intestinal epithelium interactions in the laboratory. Abstract: The intestinal epithelium is the primary interface between the host, the gut microbiome and its external environment. Since the intestinal epithelium contributes to innate immunity as a first line of defence, understanding how the epithelium responds to microbial and host stimuli is an important consideration in promoting homeostasis. Human intestinal enteroids (HIEs) are primary epithelial cell cultures that can provide insights into the biology of the intestinal epithelium and innate immune responses. One potential limitation of using HIEs for innate immune studies is the relative lack of responsiveness to factors that stimulate epithelial cytokine production. We report technical refinements, including removal of extracellular antioxidants, to facilitate enhanced cytokine responses in HIEs. Using this new method, we demonstrate that HIEs have distinct cytokine profiles in response to pro-inflammatory stimuli derived from host and microbial sources. Overall, we found that host-derived cytokines tumour necrosis factor and interleukin-1α stimulated reactive oxygen species and a large repertoire of cytokines. In contrast, microbial lipopolysaccharide, lipoteichoic acid and flagellin stimulated a limited number of cytokines and histamine did not stimulate the release of any cytokines. Importantly, HIE-secreted cytokines were functionally active, as denoted by the ability of human blood-derived neutrophil to migrate towards HIE supernatant containing interleukin-8. These findings establish that the immune responsiveness of HIEs depends on medium composition and stimuli. By refining the experimental culture medium and creating an environment conducive to epithelial cytokine responses by human enteroids, HIEs can facilitate exploration of many experimental questions pertaining to the role of the intestinal epithelium in innate immunity.

KW - cytokine

KW - flagellin

KW - histamine

KW - human intestinal enteroids (HIEs)

KW - toll-like receptors (TLR)

KW - tumor necrosis factor (TNF)

KW - Intestinal Mucosa

KW - Intestines

KW - Jejunum

KW - Humans

KW - Epithelial Cells

KW - Immunity, Innate

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DO - 10.1113/JP279423

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SP - 3085

EP - 3105

JO - Journal of Physiology

JF - Journal of Physiology

IS - 15

ER -

Enhancing responsiveness of human jejunal enteroids to host and microbial stimuli

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