Sun Yan, Keay Susan, Lehrfeld Todd J, Chai Toby C
Department of Surgery, Division of Urology, Veterans Affairs Maryland Healthcare System, University of Maryland School of Medicine, Baltimore, Maryland 2120, USA.
Urology. 2009 Nov;74(5):1163-8. doi: 10.1016/j.urology.2009.02.066. Epub 2009 Jul 22.
To determine whether antiproliferative factor (APF) or epidermal growth factor (EGF) can induce changes in purinergic signaling in normal bladder urothelial cells (BUCs) and/or whether antagonizing EGF activity or blocking adenosine triphosphate (ATP)-purinergic receptors can induce changes in purinergic signaling in interstitial cystitis (IC) cells.
IC and normal BUCs were obtained from patients' bladder biopsy specimens. IC BUCs were treated with genistein, which antagonizes EGF's activity, and normal BUCs were treated with EGF, mock APF, or APF. Suramin, which antagonizes ATP activity, was used to treat the APF-treated normal BUCs. ATP release was determined by stimulating the BUCs with 30 microM ATP and then collecting the supernatant for a 3-hour period. ATP quantification was measured by luciferin-luciferase assay. Purinergic receptor P2X, ligand-gated ion channel, 3 (P2X3) expression on BUCs was determined by fluorescence-activated cell sorting.
Genistein treatment of IC BUCs resulted in significantly decreased ATP release, thus reverting IC cells to a normal purinergic signaling phenotype. Conversely, normal BUCs treated with EGF or APF resulted in significantly increased ATP release and P2X3 expression, converting normal BUCs to an IC phenotype. Also, suramin treatment of APF-treated normal BUCs significantly reduced ATP release.
Genistein and suramin reversed the augmented ATP release in IC BUCs and APF-treated normal BUCs, respectively, suggesting the possibility of intravesical use of these agents in IC treatment. EGF and APF induced augmented purinergic signaling in normal BUCs, as determined by increased ATP release and increased P2X3 expression. These data suggest an association between cytokines and purinergic signaling in human BUCs that should be explored further.
确定抗增殖因子(APF)或表皮生长因子(EGF)是否能诱导正常膀胱尿路上皮细胞(BUCs)中嘌呤能信号的变化,和/或拮抗EGF活性或阻断三磷酸腺苷(ATP)-嘌呤能受体是否能诱导间质性膀胱炎(IC)细胞中嘌呤能信号的变化。
从患者膀胱活检标本中获取IC和正常BUCs。用拮抗EGF活性的染料木黄酮处理IC BUCs,用EGF、模拟APF或APF处理正常BUCs。用拮抗ATP活性的苏拉明处理经APF处理的正常BUCs。通过用30微摩尔ATP刺激BUCs,然后在3小时内收集上清液来测定ATP释放。通过荧光素-荧光素酶测定法测量ATP定量。通过荧光激活细胞分选法测定BUCs上嘌呤能受体P2X,配体门控离子通道,3(P2X3)的表达。
用染料木黄酮处理IC BUCs导致ATP释放显著减少,从而使IC细胞恢复到正常嘌呤能信号表型。相反,用EGF或APF处理正常BUCs导致ATP释放和P2X3表达显著增加,将正常BUCs转变为IC表型。此外,用苏拉明处理经APF处理的正常BUCs显著降低了ATP释放。
染料木黄酮和苏拉明分别逆转了IC BUCs和经APF处理的正常BUCs中增加的ATP释放,提示这些药物膀胱内使用治疗IC的可能性。如通过增加的ATP释放和增加的P2X3表达所确定的,EGF和APF在正常BUCs中诱导了增强的嘌呤能信号。这些数据表明人BUCs中细胞因子与嘌呤能信号之间存在关联,应进一步探索。