PTPN2 Regulates Interactions Between Macrophages and Intestinal Epithelial Cells to Promote Intestinal Barrier Function

被引:90
作者
Spalinger, Marianne R. [1 ]
Sayoc-Becerra, Anica [1 ]
Santos, Alina N. [1 ]
Shawki, Ali [1 ]
Canale, Vinicius [1 ]
Krishnan, Moorthy [1 ]
Niechcial, Anna [2 ,3 ]
Obialo, Nicole [2 ,3 ]
Scharl, Michael [2 ,3 ]
Li, Jiang [1 ]
Nair, Meera G. [1 ]
McCole, Declan F. [1 ]
机构
[1] Univ Calif Riverside, Div Biomed Sci, 307 Sch Med Res Bldg,900 Univ Ave, Riverside, CA 92521 USA
[2] Univ Hosp Zurich, Dept Gastroenterol & Hepatol, Zurich, Switzerland
[3] Univ Zurich, Zurich, Switzerland
基金
瑞士国家科学基金会; 美国国家卫生研究院;
关键词
TCPTP; Innate Immune Cells; Tight Junction; Claudin-2; PROTEIN-TYROSINE-PHOSPHATASE; CLAUDIN-2; EXPRESSION; TIGHT; ACTIVATION; INFLAMMATION; INDUCTION; TOLERANCE;
D O I
10.1053/j.gastro.2020.07.004
中图分类号
R57 [消化系及腹部疾病];
学科分类号
摘要
BACKGROUND & AIMS: The mechanisms by which macrophages regulate intestinal epithelial cell ( IEC) barrier properties are poorly understood. Protein tyrosine phosphatase non-receptor type 2 (PTPN2) protects the IEC barrier from inflammation- induced disruption and regulates macrophage functions. We investigated whether PTPN2 controls interactions between IECs and macrophages to maintain intestinal barrier function. METHODS: Human IEC (Caco-2BBe/HT- 29.cl19a cells) and mouse enteroid monolayers were cocultured with human macrophages (THP-1, U937, primary monocyte- derived macrophages from patients with inflammatory bowel disease [IBD]) or mouse macrophages, respectively. We assessed barrier function (transepithelial electrical resistance [TEER] and permeability to 4-kDa fluorescently labeled dextran or 70-kDa rhodamine B-dextran) and macrophage polarization. We analyzed intestinal tissues from mice with myeloid cell-specific deletion of PTPN2 (Ptpn2-LysMCre mice) and mice without disruption of Ptpn2 (controls); some mice were given injections of a neutralizing antibody against interleukin (IL) 6. Proteins were knocked down in macrophages and/or IECs with small hairpin RNAs. RESULTS: Knockdown of PTPN2 in either macrophages and/or IECs increased the permeability of IEC monolayers, had a synergistic effect when knocked down from both cell types, and increased the development of inflammatory macrophages in macrophage-IEC cocultures. Colon lamina propria from Ptpn2-LysMCre mice had significant increases in inflammatory macrophages; these mice had increased in vivo and ex vivo colon permeability to 4-kDa fluorescently labeled dextran and reduced ex vivo colon TEER. Nanostring analysis showed significant increases in the expression of IL6 in colon macrophages from Ptpn2-LysMCre mice. An IL6-blocking antibody reversed the effects of PTPN2- deficient macrophages, reducing the permeability of IEC monolayers in culture and in Ptpn2-LysMCre mice. Macrophages from patients with IBD carrying a single- nucleotide polymorphism associated with the disease ( PTPN2 rs1893217) had the same features of PTPN2-deficient macrophages from mice, including reduced TEER and increased permeability in cocultures with human IEC or mouse enteroid monolayers, which were restored by anti-IL6. CONCLUSIONS: PTPN2 is required for interactions between macrophages and IECs; loss of PTPN2 from either cell type results in intestinal barrier defects, and loss from both cell types has a synergistic effect. We provide a mechanism by which the PTPN2 gene variants compromise intestinal epithelial barrier function and increase the risk of inflammatory disorders such as IBD.
引用
收藏
页码:1763 / +
页数:29
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