PubMed:30975214 JSONTXT

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    PubMed_ArguminSci

    {"project":"PubMed_ArguminSci","denotations":[{"id":"T1","span":{"begin":124,"end":258},"obj":"DRI_Challenge"},{"id":"T2","span":{"begin":259,"end":386},"obj":"DRI_Background"},{"id":"T3","span":{"begin":387,"end":598},"obj":"DRI_Background"},{"id":"T4","span":{"begin":599,"end":693},"obj":"DRI_Background"},{"id":"T5","span":{"begin":694,"end":841},"obj":"DRI_Background"},{"id":"T6","span":{"begin":842,"end":1068},"obj":"DRI_Approach"},{"id":"T7","span":{"begin":1069,"end":1162},"obj":"DRI_Background"},{"id":"T8","span":{"begin":1163,"end":1246},"obj":"DRI_Background"},{"id":"T9","span":{"begin":1247,"end":1358},"obj":"DRI_Background"},{"id":"T10","span":{"begin":1359,"end":1450},"obj":"DRI_Background"},{"id":"T11","span":{"begin":1451,"end":1594},"obj":"DRI_Approach"},{"id":"T12","span":{"begin":1595,"end":1691},"obj":"DRI_Outcome"}],"text":"Bovine fetal mesenchymal stem cells exert antiproliferative effect against mastitis causing pathogen Staphylococcus aureus.\nStaphylococcus aureus is the most commonly isolated pathogen from clinical bovine mastitis samples and a difficult pathogen to combat. Mesenchymal stem cells (MSC) are multipotent progenitor cells equipped with a variety of factors that inhibit bacterial growth. The aim of the present study was to evaluate the in vitro antibacterial potential against S. aureus of conditioned medium (CM) from MSC derived from fetal bovine bone marrow (BM-MSC) and adipose tissue (AT-MSC). BM-MSC, AT-MSC and fetal fibroblasts (FB) cultures were activated by infection with S. aureus. Bacterial growth was evaluated in presence of CM, concentrated CM (CCM), activated CM (ACM) and concentrated ACM (CACM) from BM-MSC, AT-MSC and FB. Gene expression of β-defensin 4A (bBD-4A), NK-lysine 1 (NK1), cathelicidin 2 (CATHL2), hepcidin (HEP) and indoleamine 2,3 dioxygenase (IDO) and protein expression of bBD-4A were determined in activated and non-activated cells. The majority of BM-MSC and AT-MSC expressed CD73, Oct4 and Nanog, and were negative for CD34. Growth of S. aureus decreased when it was exposed to CM from BM-MSC, AT-MSC and FB. Moreover, growth of S. aureus in CCM, ACM and CACM was lower compared to controls of CM from BM-MSC and AT-MSC. Activated AT-MSC increased mRNA levels of bBD4A and NK1, and protein levels of bBD4A in CM. Thus, CM from fetal bovine BM-MSC and AT-MSC has the capacity to reduce in average ~30% of S. aureus relative growth under in vitro conditions. The in vitro antibacterial effect of fetal bovine MSC may be mediated by bBD4A and NK1 activity."}

    Goldhamster2_Cellosaurus

    {"project":"Goldhamster2_Cellosaurus","denotations":[{"id":"T1","span":{"begin":227,"end":228},"obj":"CVCL_6479|Finite_cell_line|Mus musculus"},{"id":"T2","span":{"begin":335,"end":336},"obj":"CVCL_6479|Finite_cell_line|Mus musculus"},{"id":"T3","span":{"begin":510,"end":512},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T4","span":{"begin":542,"end":560},"obj":"CVCL_4399|Finite_cell_line|Bos taurus"},{"id":"T5","span":{"begin":562,"end":564},"obj":"CVCL_E481|Transformed_cell_line|Homo sapiens"},{"id":"T6","span":{"begin":562,"end":564},"obj":"CVCL_S926|Spontaneously_immortalized_cell_line|Lates calcarifer"},{"id":"T7","span":{"begin":599,"end":601},"obj":"CVCL_E481|Transformed_cell_line|Homo sapiens"},{"id":"T8","span":{"begin":599,"end":601},"obj":"CVCL_S926|Spontaneously_immortalized_cell_line|Lates calcarifer"},{"id":"T9","span":{"begin":655,"end":664},"obj":"CVCL_C410|Hybridoma|Mus musculus"},{"id":"T10","span":{"begin":740,"end":742},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T11","span":{"begin":757,"end":759},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T12","span":{"begin":761,"end":764},"obj":"CVCL_2613|Cancer_cell_line|Homo sapiens"},{"id":"T13","span":{"begin":761,"end":764},"obj":"CVCL_R825|Spontaneously_immortalized_cell_line|Labeo catla"},{"id":"T14","span":{"begin":761,"end":764},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T15","span":{"begin":767,"end":776},"obj":"CVCL_C410|Hybridoma|Mus musculus"},{"id":"T16","span":{"begin":777,"end":779},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T17","span":{"begin":819,"end":821},"obj":"CVCL_E481|Transformed_cell_line|Homo sapiens"},{"id":"T18","span":{"begin":819,"end":821},"obj":"CVCL_S926|Spontaneously_immortalized_cell_line|Lates calcarifer"},{"id":"T19","span":{"begin":885,"end":887},"obj":"CVCL_1D01|Cancer_cell_line|Rattus norvegicus"},{"id":"T20","span":{"begin":1034,"end":1043},"obj":"CVCL_C410|Hybridoma|Mus musculus"},{"id":"T21","span":{"begin":1052,"end":1061},"obj":"CVCL_C410|Hybridoma|Mus musculus"},{"id":"T22","span":{"begin":1085,"end":1087},"obj":"CVCL_E481|Transformed_cell_line|Homo sapiens"},{"id":"T23","span":{"begin":1085,"end":1087},"obj":"CVCL_S926|Spontaneously_immortalized_cell_line|Lates calcarifer"},{"id":"T24","span":{"begin":1216,"end":1218},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T25","span":{"begin":1224,"end":1226},"obj":"CVCL_E481|Transformed_cell_line|Homo sapiens"},{"id":"T26","span":{"begin":1224,"end":1226},"obj":"CVCL_S926|Spontaneously_immortalized_cell_line|Lates calcarifer"},{"id":"T27","span":{"begin":1280,"end":1283},"obj":"CVCL_2613|Cancer_cell_line|Homo sapiens"},{"id":"T28","span":{"begin":1280,"end":1283},"obj":"CVCL_R825|Spontaneously_immortalized_cell_line|Labeo catla"},{"id":"T29","span":{"begin":1280,"end":1283},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T30","span":{"begin":1332,"end":1334},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T31","span":{"begin":1340,"end":1342},"obj":"CVCL_E481|Transformed_cell_line|Homo sapiens"},{"id":"T32","span":{"begin":1340,"end":1342},"obj":"CVCL_S926|Spontaneously_immortalized_cell_line|Lates calcarifer"},{"id":"T33","span":{"begin":1359,"end":1368},"obj":"CVCL_C410|Hybridoma|Mus musculus"},{"id":"T34","span":{"begin":1447,"end":1449},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T35","span":{"begin":1457,"end":1459},"obj":"CVCL_H246|Cancer_cell_line|Homo sapiens"},{"id":"T36","span":{"begin":1478,"end":1480},"obj":"CVCL_E481|Transformed_cell_line|Homo sapiens"},{"id":"T37","span":{"begin":1478,"end":1480},"obj":"CVCL_S926|Spontaneously_immortalized_cell_line|Lates calcarifer"},{"id":"T38","span":{"begin":1496,"end":1499},"obj":"CVCL_6758|Undefined_cell_line_type|Cricetulus griseus"},{"id":"T39","span":{"begin":1496,"end":1499},"obj":"CVCL_E689|Transformed_cell_line|Homo sapiens"},{"id":"T40","span":{"begin":1535,"end":1537},"obj":"CVCL_J925|Hybridoma|Mus musculus"},{"id":"T41","span":{"begin":1649,"end":1652},"obj":"CVCL_E773|Transformed_cell_line|Homo sapiens"},{"id":"T42","span":{"begin":1682,"end":1690},"obj":"CVCL_C410|Hybridoma|Mus musculus"}],"text":"Bovine fetal mesenchymal stem cells exert antiproliferative effect against mastitis causing pathogen Staphylococcus aureus.\nStaphylococcus aureus is the most commonly isolated pathogen from clinical bovine mastitis samples and a difficult pathogen to combat. Mesenchymal stem cells (MSC) are multipotent progenitor cells equipped with a variety of factors that inhibit bacterial growth. The aim of the present study was to evaluate the in vitro antibacterial potential against S. aureus of conditioned medium (CM) from MSC derived from fetal bovine bone marrow (BM-MSC) and adipose tissue (AT-MSC). BM-MSC, AT-MSC and fetal fibroblasts (FB) cultures were activated by infection with S. aureus. Bacterial growth was evaluated in presence of CM, concentrated CM (CCM), activated CM (ACM) and concentrated ACM (CACM) from BM-MSC, AT-MSC and FB. Gene expression of β-defensin 4A (bBD-4A), NK-lysine 1 (NK1), cathelicidin 2 (CATHL2), hepcidin (HEP) and indoleamine 2,3 dioxygenase (IDO) and protein expression of bBD-4A were determined in activated and non-activated cells. The majority of BM-MSC and AT-MSC expressed CD73, Oct4 and Nanog, and were negative for CD34. Growth of S. aureus decreased when it was exposed to CM from BM-MSC, AT-MSC and FB. Moreover, growth of S. aureus in CCM, ACM and CACM was lower compared to controls of CM from BM-MSC and AT-MSC. Activated AT-MSC increased mRNA levels of bBD4A and NK1, and protein levels of bBD4A in CM. Thus, CM from fetal bovine BM-MSC and AT-MSC has the capacity to reduce in average ~30% of S. aureus relative growth under in vitro conditions. The in vitro antibacterial effect of fetal bovine MSC may be mediated by bBD4A and NK1 activity."}

    GoldHamster

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fetal mesenchymal stem cells exert antiproliferative effect against mastitis causing pathogen Staphylococcus aureus.\nStaphylococcus aureus is the most commonly isolated pathogen from clinical bovine mastitis samples and a difficult pathogen to combat. Mesenchymal stem cells (MSC) are multipotent progenitor cells equipped with a variety of factors that inhibit bacterial growth. The aim of the present study was to evaluate the in vitro antibacterial potential against S. aureus of conditioned medium (CM) from MSC derived from fetal bovine bone marrow (BM-MSC) and adipose tissue (AT-MSC). BM-MSC, AT-MSC and fetal fibroblasts (FB) cultures were activated by infection with S. aureus. Bacterial growth was evaluated in presence of CM, concentrated CM (CCM), activated CM (ACM) and concentrated ACM (CACM) from BM-MSC, AT-MSC and FB. Gene expression of β-defensin 4A (bBD-4A), NK-lysine 1 (NK1), cathelicidin 2 (CATHL2), hepcidin (HEP) and indoleamine 2,3 dioxygenase (IDO) and protein expression of bBD-4A were determined in activated and non-activated cells. The majority of BM-MSC and AT-MSC expressed CD73, Oct4 and Nanog, and were negative for CD34. Growth of S. aureus decreased when it was exposed to CM from BM-MSC, AT-MSC and FB. Moreover, growth of S. aureus in CCM, ACM and CACM was lower compared to controls of CM from BM-MSC and AT-MSC. Activated AT-MSC increased mRNA levels of bBD4A and NK1, and protein levels of bBD4A in CM. Thus, CM from fetal bovine BM-MSC and AT-MSC has the capacity to reduce in average ~30% of S. aureus relative growth under in vitro conditions. The in vitro antibacterial effect of fetal bovine MSC may be mediated by bBD4A and NK1 activity."}