Nakada S Y, Saban R, Zine M J, Uehling D T, Bjorling D E
Department of Surgery, University of Wisconsin Medical School, Madison, USA.
J Urol. 1998 Nov;160(5):1924-7.
To develop an in vitro model of passive sensitization for the ureter for the study of noninfectious ureteral inflammation.
Human ureteral tissues were obtained from excess segments of ureters from patients undergoing donor nephrectomy. Following excision, ureters were placed in physiologic salt solution (PSS) and passively sensitized by incubating with ragweed serum from allergic donor (1 ml. serum: 4 ml. PSS) for 20 hours at room temperature. Ureteral segments were incubated with PSS only and served as non-sensitized controls (n = 4). After sensitization, excess serum was removed by serial washing with PSS without serum. Ureteral strips were then suspended in vitro for determination of tissue contraction. Contractile responses and histamine release were measured. Tissues were then exposed to antigen. To investigate the role of inflammatory mediators in tissue contraction, 4 groups of 8 sensitized ureteral segments were incubated for 1 hour with the following substances: a H1 histamine receptor antagonist (pyrilamine), an inhibitor of prostaglandin synthesis (indomethacin), an inhibitor of leukotriene synthesis (A-64077), and a control substance (DMSO). Following incubation, the tissues were exposed to antigen, and contraction and histamine release were determined.
Sensitized ureteral segments (n = 8) responded to antigen with contraction (30% BaCl maximum; p <0.01) and histamine release (205/ng./gm. tissue) within the first 5 minutes of superfusion. Non-sensitized control segments (n = 4) did not respond. Both indomethacin and pyrilamine reduced (7-10% of BaCl maximum; p <0.05) the contractile response of sensitized ureter to antigen, whereas A-64077 did not. Analysis of the superfusate for histamine indicates that indomethacin reduced histamine release (150 ng./gm.) whereas A-64077 and pyrilamine did not (p <0.05).
We have demonstrated that ureteral segments can be passively sensitized and that subsequent antigen challenge stimulates contraction and histamine release. Our findings suggest that contraction of ureteral tissue and histamine release may be utilized as an inherent bioassay indicating the activity of inflammatory mediators. In addition, these results suggest that both prostaglandins and histamine, but apparently not leukotrienes, participate in the early inflammatory response to antigen challenge of the sensitized ureter.
建立输尿管被动致敏的体外模型,用于研究非感染性输尿管炎症。
从接受供体肾切除术患者多余的输尿管段获取人输尿管组织。切除后,将输尿管置于生理盐溶液(PSS)中,并在室温下与来自过敏供体的豚草血清(1毫升血清:4毫升PSS)孵育20小时进行被动致敏。仅用PSS孵育输尿管段作为未致敏对照(n = 4)。致敏后,通过用无血清PSS连续洗涤去除多余血清。然后将输尿管条带体外悬置以测定组织收缩。测量收缩反应和组胺释放。然后使组织暴露于抗原。为研究炎症介质在组织收缩中的作用,将4组每组8个致敏输尿管段与以下物质孵育1小时:一种H1组胺受体拮抗剂(吡苄明)、一种前列腺素合成抑制剂(吲哚美辛)、一种白三烯合成抑制剂(A - 64077)和一种对照物质(二甲亚砜)。孵育后,使组织暴露于抗原,并测定收缩和组胺释放。
致敏输尿管段(n = 8)在灌注的前5分钟内对抗原产生收缩反应(最大BaCl的30%;p <0.01)和组胺释放(205纳克/克组织)。未致敏对照段(n = 4)无反应。吲哚美辛和吡苄明均降低了(最大BaCl的7 - 10%;p <0.05)致敏输尿管对抗原的收缩反应,而A - 64077未降低。对灌注液中的组胺分析表明,吲哚美辛减少了组胺释放(150纳克/克),而A - 64077和吡苄明未减少(p <0.05)。
我们已证明输尿管段可被被动致敏,且随后的抗原刺激会引发收缩和组胺释放。我们的研究结果表明,输尿管组织的收缩和组胺释放可作为一种内在生物测定方法来指示炎症介质的活性。此外,这些结果表明前列腺素和组胺,但显然不是白三烯,参与了致敏输尿管对抗原刺激的早期炎症反应。
