Diamond Michael P, Kruger Michael, Saed Ghassan M
Department of Obstetrics and Gynecology, Wayne State University/Detroit Medical Center, Detroit, Michigan, USA.
Fertil Steril. 2004 Jun;81(6):1657-64. doi: 10.1016/j.fertnstert.2003.12.022.
To examine the effect of fibrin sealant on mRNA expression of factors regulating plasminogen activator activity in human peritoneal cells. Plasminogen activator activity is thought to play a pivotal role in degradation of the proteinaceous mass that develops after surgical procedures. Reduction of plasminogen activator activity, as occurs with tissue trauma, results in increased postoperative adhesion development.
Tissue culture for 6, 12, 24, and 48 hours.
University research laboratory.
Source of mesothelial cells with fibroblasts.
INTERVENTION(S): Measurement of mRNA expression of tissue plasminogen activator (t-PA) and plasminogen activator inhibitor 1 (PAI-1).
MAIN OUTCOME MEASURE(S): Multiplex reverse transcriptase/polymerase chain reaction (RT/PCR) was used to determine relative change in t-PA and PAI-1 mRNA levels under six conditions: [1]. fibrin sealant (Tisseel); [2]. fibrin sealant (Tisseel) two components diluted 1:2; [3]. fibrin sealant (Tisseel) sealer protein component reconstituted without aprotinin (a protease inhibitor); [4]. fibrin sealant (Tisseel) sealer protein component reconstituted without aprotinin, both components diluted 1:2; [5]. fibrin sealant (Tisseel) components diluted to physiologic concentrations; and [6] control (culture media).
The mRNA levels of t-PA and PAI-1 by human peritoneal cells were unchanged during 48 hours. In mesothelial cells, the addition of the compositions increased t-PA mRNA levels. A selective increase was observed in the normal peritoneal fibroblasts at the later time points; similar increases were identified in adhesion fibroblast cultures. In mesothelial cells, the more concentrated compositions generally increased PAI-1 mRNA above control levels, whereas in normal peritoneal fibroblasts PAI-1 levels generally remained unchanged. In contrast, in adhesion fibroblasts, PAI-1 levels decreased over time with treatment.
CONCLUSION(S): Fibrin sealant, in the presence and absence of aprotinin, increases both t-PA and PAI-1 expression by human peritoneal cells; changes not seen with physiologic concentrations of fibrin sealant. These observations suggest that in addition to its ability to help achieve hemostasis, fibrin sealant affects the healing process by altering components of the plasminogen activator system, which may be of benefit in the reduction of postoperative adhesions.
研究纤维蛋白封闭剂对人腹膜细胞中调节纤溶酶原激活物活性的因子mRNA表达的影响。纤溶酶原激活物活性被认为在手术操作后形成的蛋白质团块的降解过程中起关键作用。组织创伤时纤溶酶原激活物活性降低,会导致术后粘连增加。
进行6、12、24和48小时的组织培养。
大学研究实验室。
间皮细胞与成纤维细胞的来源。
测量组织型纤溶酶原激活物(t-PA)和纤溶酶原激活物抑制剂1(PAI-1)的mRNA表达。
采用多重逆转录/聚合酶链反应(RT/PCR)测定在六种条件下t-PA和PAI-1 mRNA水平的相对变化:[1]纤维蛋白封闭剂(Tisseel);[2]纤维蛋白封闭剂(Tisseel)的两种成分按1:2稀释;[3]纤维蛋白封闭剂(Tisseel)的封闭蛋白成分在无抑肽酶(一种蛋白酶抑制剂)的情况下重构;[4]纤维蛋白封闭剂(Tisseel)的封闭蛋白成分在无抑肽酶的情况下重构,两种成分均按1:2稀释;[5]纤维蛋白封闭剂(Tisseel)的成分稀释至生理浓度;[6]对照(培养基)。
人腹膜细胞的t-PA和PAI-1 mRNA水平在48小时内未发生变化。在间皮细胞中,添加这些组合物可增加t-PA mRNA水平。在后期时间点,正常腹膜成纤维细胞中观察到选择性增加;在粘连成纤维细胞培养物中也发现了类似的增加。在间皮细胞中,浓度较高的组合物通常使PAI-1 mRNA水平高于对照水平,而在正常腹膜成纤维细胞中,PAI-1水平通常保持不变。相比之下,在粘连成纤维细胞中,随着治疗时间的延长,PAI-1水平下降。
无论有无抑肽酶,纤维蛋白封闭剂均可增加人腹膜细胞中t-PA和PAI-1的表达;生理浓度的纤维蛋白封闭剂未见此变化。这些观察结果表明,纤维蛋白封闭剂除了具有帮助实现止血的能力外,还通过改变纤溶酶原激活物系统的成分来影响愈合过程,这可能有助于减少术后粘连。
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