Systemic and intestinal levels of factor XIII-A: the impact of inflammation on expression in macrophage subtypes

被引:15
作者
Soendergaard, Christoffer [1 ,2 ]
Kvist, Peter Helding [2 ]
Seidelin, Jakob Benedict [1 ]
Pelzer, Hermann [3 ]
Nielsen, Ole Haagen [1 ]
机构
[1] Univ Copenhagen, Herlev Hosp, Med Sect, Dept Gastroenterol 54O3, Herlev Ringvej 75, DK-2730 Herlev, Denmark
[2] Novo Nordisk AS, Dept Histol & Bioimaging, Malov, Denmark
[3] Novo Nordisk AS, Dept Res Bioanal, Malov, Denmark
关键词
Factor XIII; Immunohistochemistry; Inflammation; In situ hybridization; Macrophages; Ulcerative colitis; COAGULATION-FACTOR-XIII; ULCERATIVE-COLITIS; CROHNS-DISEASE; BOWEL-DISEASE; DENDRITIC CELLS; B SUBUNITS; TRANSGLUTAMINASE; ACTIVATION; PARAMETERS; MONOCYTE;
D O I
10.1007/s00535-015-1152-2
中图分类号
R57 [消化系及腹部疾病];
学科分类号
摘要
Subunit A of coagulation factor XIII (FXIII-A) is important for clot stability and acts in the subsequent wound healing process. Loss of plasma FXIII-A has been reported after surgery, sepsis, and inflammatory conditions. In the intestinal mucosa, FXIII-A is expressed by macrophages and cellular FXIII-A has been associated with phagocytosis and migration of macrophages. The objective was to evaluate the consequences of intestinal inflammation on resident mucosal macrophages, focusing on the level and distribution of FXIII-A. Plasma and colonic biopsies were collected from 67 patients with ulcerative colitis and controls. Intestinal samples were stained using immunohistochemistry for FXIII-A and macrophages (CD68, CD163 and iNOS). In situ hybridization were used to assess the intestinal expression of FXIII-A. FXIII-A antigen and activity levels were measured in plasma. Increased infiltration of CD68 positive macrophages in the inflamed mucosa coincided with increased extracellular deposited FXIII-A and decreased expression and intracellular protein levels of FXIII-A. A decreased proportion of FXIII-A/CD68/CD163 triple-positive macrophages was observed in inflamed mucosa, indicating a reduction of the M2 phenotype with consequent loss of FXIII-A. No induction of iNOS positive macrophages was observed. Stimulation of na < ve monocytes with physiological concentrations of pro-inflammatory mediators negatively affected the expression of FXIII-A. Measurements in plasma confirmed the loss of both FXIII antigen and activity during active disease. Intestinal inflammation in UC induces loss of M2 macrophages with subsequent loss of FXIII-A synthesis. The loss of cellular FXIII-A may impact migration and phagocytosis, and hence limit pathogen eradication in UC.
引用
收藏
页码:796 / 807
页数:12
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