Molecular Profile of Barrett's Esophagus and Gastroesophageal Reflux Disease in the Development of Translational Physiological and Pharmacological Studies

被引:8
作者
Korbut, Edyta [1 ]
Janmaat, Vincent T. [2 ]
Wierdak, Mateusz [1 ,3 ]
Hankus, Jerzy [4 ]
Wojcik, Dagmara [1 ]
Surmiak, Marcin [1 ,5 ]
Magierowska, Katarzyna [1 ]
Brzozowski, Tomasz [1 ]
Peppelenbosch, Maikel P. [2 ]
Magierowski, Marcin [1 ]
机构
[1] Jagiellonian Univ, Dept Physiol, Med Coll, PL-31531 Krakow, Poland
[2] Erasmus MC, Dept Gastroenterol & Hepatol, Univ Med Ctr Rotterdam, NL-3015 CN Rotterdam, Netherlands
[3] Jagiellonian Univ, Dept Gen Surg 2, Med Coll, PL-30688 Krakow, Poland
[4] Jagiellonian Univ, Dept Pathomorphol, Med Coll, PL-31531 Krakow, Poland
[5] Jagiellonian Univ, Dept Internal Med, Med Coll, PL-31066 Krakow, Poland
关键词
Barrett's esophagus; esophageal epithelium; molecular profile; molecular gastrointestinal pharmacology; molecular gastrointestinal pathophysiology; EPIDERMAL-GROWTH-FACTOR; EPITHELIAL-CELLS; ANIMAL-MODEL; ADENOCARCINOMA; METAPLASIA; CYCLOOXYGENASE-2; CARCINOGENESIS; PROLIFERATION; PROGRESSION; EXPRESSION;
D O I
10.3390/ijms21176436
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Barrett's esophagus (BE) is a premalignant condition caused by gastroesophageal reflux disease (GERD), where physiological squamous epithelium is replaced by columnar epithelium. Several in vivo and in vitro BE models were developed with questionable translational relevance when implemented separately. Therefore, we aimed to screen Gene Expression Omnibus 2R (GEO2R) databases to establish whether clinical BE molecular profile was comparable with animal and optimized human esophageal squamous cell lines-based in vitro models. The GEO2R tool and selected databases were used to establish human BE molecular profile. BE-specific mRNAs in human esophageal cell lines (Het-1A and EPC2) were determined after one, three and/or six-day treatment with acidified medium (pH 5.0) and/or 50 and 100 mu M bile mixture (BM). Wistar rats underwent microsurgical procedures to generate esophagogastroduodenal anastomosis (EGDA) leading to BE. BE-specific genes (keratin (KRT)1,KRT4,KRT5,KRT6A,KRT13,KRT14,KRT15,KRT16,KRT23, KRT24,KRT7,KRT8,KRT18,KRT20, trefoil factor (TFF)1,TFF2,TFF3, villin (VIL)1, mucin (MUC)2,MUC3A/B,MUC5B,MUC6andMUC13) mRNA expression was assessed by real-time PCR. Pro/anti-inflammatory factors (interleukin (IL)-1 beta, IL-2, IL-4, IL-5, IL-6, IL-10, IL-12, IL-13, tumor necrosis factor alpha, interferon gamma, granulocyte-macrophage colony-stimulating factor) serum concentration was assessed by a Luminex assay. Expression profile in vivo reflected about 45% of clinical BE with accompanied inflammatory response. Six-day treatment with 100 mu M BM (pH 5.0) altered gene expression in vitro reflecting in 73% human BE profile and making this the most reliable in vitro tool taking into account two tested cell lines. Our optimized and established combined in vitro and in vivo BE models can improve further physiological and pharmacological studies testing pathomechanisms and novel therapeutic targets of this disorder.
引用
收藏
页码:1 / 27
页数:26
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