Woo J, Lemster B, Tamura K, Starzl T E, Thomson A W
Transplant Institute, University of Pittsburgh Health Science Center, Pennsylvania 15213.
Transplantation. 1993 Aug;56(2):374-81. doi: 10.1097/00007890-199308000-00024.
Based on its capacity to inhibit de novo pyrimidine biosynthesis by blocking dihydroorotate dehydrogenase activity, the antitumor agent brequinar sodium (BQR) has emerged as a new immunosuppressive agent. Since BQR is known to prevent the synthesis of nucleotides during cell proliferation, we hypothesized that it would be highly effective in controlling strong lymphocyte proliferative responses but might be less effective in controlling comparatively weak responses that do not necessarily involve new nucleotide synthesis. We addressed this question by culturing murine spleen cells with different types of stimuli, including Con A, phorbol myristate acetate +/- ionomycin, anti-CD3, and anti-Igs. Addition of BQR (0.001 microgram/ml to 10 micrograms/ml) at the start of a 72-hr culture period caused dose-dependent inhibition of strong proliferative responses, induced either by Con A (5 micrograms/ml) or PMA+ionomycin. A residual degree of proliferation persisted, however, even at the highest BQR concentrations. In contrast, no impairment of low-concentration Con A (0.5 or 0.1 microgram/ml), anti-CD3, or anti-Igs responses was observed. In order to ascertain its role in arresting nucleotide synthesis, we attempted to reverse the inhibitory effect of BQR by adding exogenous uridine or cytidine to lymphocyte cultures. BQR's inhibitory activity was reversed completely by adding uridine at 0.1 mM. In contrast, combination of BQR and cytidine (0.1 mM) potentiated BQR's activity and abrogated anti-CD3 or anti-Igs-induced lymphocyte proliferation in a dose-dependent manner. A synergistic inhibitory action between BQR and cytidine was observed when the BQR concentration was higher than 0.1 microgram/ml and with cytidine at 0.1 mM. Production of interleukin-2 and IL-4 was only slightly affected by BQR, but was significantly suppressed by coadministration of BQR and cytidine. Neither BQR (5 micrograms/ml) on its own, however, nor combination of BQR with cytidine affected production of mRNA for IL-2, IL-4, or interferon-gamma, as determined by reverse-transcription polymerase chain reaction. Our observations suggest that BQR may not only affect dihydroorotate dehydrogenase activity, but may also inhibit the enzyme cytidine deaminase, which converts cytidine to uridine. These antimetabolic effects of BQR complement the well-known cytokine synthesis inhibitory actions of FK506 or CsA. The combination of BQR and cytidine, however, offers a further possibility for inhibition of both cytokine production and T and B cell proliferation, and may have potential for the control of graft rejection.
基于其通过阻断二氢乳清酸脱氢酶活性抑制嘧啶从头生物合成的能力,抗肿瘤药物布喹那钠(BQR)已成为一种新型免疫抑制剂。由于已知BQR可在细胞增殖过程中阻止核苷酸的合成,我们推测它在控制强烈的淋巴细胞增殖反应方面可能非常有效,但在控制不一定涉及新核苷酸合成的相对较弱反应方面可能效果较差。我们通过用不同类型的刺激物培养小鼠脾细胞来解决这个问题,这些刺激物包括刀豆蛋白A(Con A)、佛波酯肉豆蔻酸酯+/-离子霉素、抗CD3和抗免疫球蛋白(anti-Igs)。在72小时培养期开始时添加BQR(0.001微克/毫升至10微克/毫升)会导致由Con A(5微克/毫升)或佛波酯(PMA)+离子霉素诱导的强烈增殖反应受到剂量依赖性抑制。然而,即使在最高BQR浓度下,仍有一定程度的增殖残留。相比之下,未观察到低浓度Con A(0.5或0.1微克/毫升)、抗CD3或抗Igs反应受到损害。为了确定其在阻止核苷酸合成中的作用,我们试图通过向淋巴细胞培养物中添加外源性尿苷或胞苷来逆转BQR的抑制作用。添加0.1 mM尿苷可完全逆转BQR的抑制活性。相比之下,BQR与胞苷(0.1 mM)的组合增强了BQR的活性,并以剂量依赖性方式消除了抗CD3或抗Igs诱导的淋巴细胞增殖。当BQR浓度高于0.1微克/毫升且胞苷浓度为0.1 mM时,观察到BQR与胞苷之间存在协同抑制作用。白细胞介素-2(IL-2)和IL-4的产生仅受到BQR的轻微影响,但BQR与胞苷共同给药可显著抑制其产生。然而,通过逆转录聚合酶链反应测定,单独的BQR(5微克/毫升)或BQR与胞苷的组合均未影响IL-2、IL-4或干扰素-γ的mRNA产生。我们的观察结果表明,BQR可能不仅影响二氢乳清酸脱氢酶的活性,还可能抑制将胞苷转化为尿苷的胞苷脱氨酶。BQR的这些抗代谢作用补充了众所周知的FK506或环孢素A(CsA)的细胞因子合成抑制作用。然而,BQR与胞苷的组合为抑制细胞因子产生以及T和B细胞增殖提供了进一步的可能性,并且可能在控制移植排斥方面具有潜力。
