CN1148350C - 新型VLA-4抑制剂:oMePUPA-V - Google Patents
新型VLA-4抑制剂:oMePUPA-V Download PDFInfo
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- CN1148350C CN1148350C CNB998080020A CN99808002A CN1148350C CN 1148350 C CN1148350 C CN 1148350C CN B998080020 A CNB998080020 A CN B998080020A CN 99808002 A CN99808002 A CN 99808002A CN 1148350 C CN1148350 C CN 1148350C
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Abstract
本发明公开了一种细胞粘着抑制剂oMePUPA-V,(R)-N-[[4-[[(2-甲基苯基氨基)羰基]氨基]苯基]乙酰基]-L-脯氨酰基-3-甲基)-β-丙氨酸,药物组合物,和治疗细胞粘着介导的病状的方法。
Description
本发明涉及用于抑制、变更或预防细胞粘着和细胞粘着介导致病状的新化合物。本发明还涉及含有这些化合物的药物制剂,以及使用它们抑制和预防细胞粘着和细胞粘着介导致病的方法。可以将本发明的这些化合物和药物组合物用作治疗和预防药物。它们特别适宜治疗许多炎性和自身免疫性疾病。
细胞粘着为细胞彼此结合、向特定靶子移动或定位在胞外基质中的过程。细胞粘着本身构成许多生物现象的基本机制之一。例如,细胞粘着引起造血细胞粘附到内皮细胞上,接着这些造血细胞移到血管外并移到损伤部位。细胞粘着本身在如哺乳动物的炎症和免疫反应的许多病状中起作用。
对细胞粘着的分子基础研究显示,不同细胞表面的大分子—共同称之为粘着分子或受体—介导细胞-细胞和细胞-基质相互作用。例如,所谓“整联蛋白”的超家族蛋白质是造血细胞和其微环境之间粘附相互作用的关键介导体(M.E.Hemler,"整联蛋白家族中的VLA蛋白质:结构、功能和其对白细胞的作用"Ann.Rev.Immunol.,8,第365页(1990))。整联蛋白为非共价杂二聚体络合物,由两个所谓的α和β亚单元组成。有至少17个不同的α亚单元(α1-α10、α-L、α-M、α-D、α-X、α-IIB、α-V和α-E)和至少9个不同的β(β1-β9)亚单元,到目前为止它们都已被识别。基于其α和β亚单元组分的类型,可以将每个整联蛋白归类到亚家族中。
整联蛋白α4β1,最近也称之为抗原-4(“VLA-4”)或CD49d/CD29,为参与广泛的细胞-细胞和细胞-基质粘附相互作用的白细胞细胞表面受体(M.E.Hemler,Ann.Rev.Immunol.,8,第365页(1990))。它被充当白细胞诱导的内皮细胞表面蛋白质的受体,血管细胞粘着分子-1(“VCAM-1”),以及胞外基质蛋白质纤连蛋白(“FN”)的受体(Ruegg等人,J.Cell Biol.,177,第179页(1991));Wayner等人,
J.Cell Biol.,105,第1873页(1987);Kramer等人,
J.Biol.Chem.,264,第4684页(1989);Gehlsen等人,
Science,24,第1228页(1988))。抗-VLA-4单克隆抗体(″mAb’s″)已显示出在体外和体内都抑制VLA-4-依赖性粘着相互作用(Ferguson等人,
Proc.Natl.Acad.Sci.,88,第8072页(1991);Ferguson等人,
J.Immunol.150,第1172页(1993)).体内试验的结果暗示,抑制VLA-4-依赖性细胞粘着可以预防、抑制或改变几种炎性和自体免疫病状。(R.L.Lobb等人,″The Pathophysiologic Role of α4整联蛋白在体内的病理生理作用,94,第1722-28页(1994))。
为了鉴定结合VLA-4所必需的最小活性氨基酸序列,Komoriya等人合成了许多以特种纤连蛋白的CS-1区域(VLA-4结合域)的氨基酸序列为基础的重叠肽。(″在纤连蛋白的选择性剪接型III连接片段域中主细胞型特异性粘着位点的最小必需序列(CS1)为亮氨酸-天冬氨酸-缬氨酸″
J.Biol. Chem.,266(23).第15075-79页(1991))。它们鉴定了一8-氨基酸肽,Glu-Ile-Leu-Asp-Val-Pro-Ser-Thr,以及两个较小的重叠五肽,Glu-Ile-Leu-Asp-Val和Leu-Asp-Val-Pro-Ser,它们具有抗FN-依赖性细胞粘着的抑制活性。这些结果暗示,三肽Leu-Asp-Val是细胞粘着活性的最小序列。后来证实,Leu-Asp-Val仅结合表达VLA-4活性形式的淋巴细胞,因此使人们不相信能在体内能利用这种肽(E.A.Wayner等人,“在纤连蛋白的V区域中LDV序列的造血细胞的激活依赖性识别”,
J.Cell. Biol.,116(2),第489-497页(1992))。但是,含有LDV序列的某些较大肽后来显示出在体内有活性(T.A.Ferguson等人,“两个整联蛋白结合肽使体内的T-细胞介导免疫反应无效”,
Proc.Natl.Acad.Sci.USA,88,第8072-76页(1991);和S.M.Wahl等人,″合成纤连蛋白肽通过中断白细胞粘着和募集来抑制大鼠关节炎″,
J.Clin.Invest.,94,第655-62页(1994))。还描述了能够抑制VLA-4和VLA-5粘着到FN上的环五肽。(参见例如,D.M.Nowlin等人″新型环五肽抑制a4β1和α5β1整联蛋白介导的细胞粘着″,
J.Biol.Chem.,268(27),第20352-59页(1993);以及PCT申请PCT/US91/04862)。该五肽以来自已知为几种胞外基质蛋白质的识别位点中的常规主题的FN的三肽序列Arg-GIy-Asp为基础。
例如在未决美国专利申请08/376372和WO98/04913(在此引入作为参考)中已报道了VLA-4抑制剂的其它例子。USSN 376372描述了具有细胞粘着抑制活性的含β-氨基酸的线性肽基化合物。国际专利申请94/15958和WO92/00995(特别引入作为参考)描述了具有细胞粘着调节活性的环状肽和肽模拟化合物。国际专利申请WO93/08823和WO92/08464(本文特别引入作为参考)含有胍基、脲基和硫脲基的细胞粘着调节化合物。美国专利US5260277描述了胍基细胞粘着调节化合物,将其特别引入本文。
尽管有这些优点,但是还需要具有提高的药动学和药效性如口服生物可利用率和有效作用时间的低分子量VLA-4依赖性细胞粘着特异性抑制剂。这些化合物将提供对治疗、改变、预防或抑制通过细胞粘着和VLA-4结合所介导的各种病状有用的药物。
本发明的化合物为VLA-4整联蛋白抑制剂,因此阻断VLA-4结合到其各种配体上,如VCAM-1和纤连蛋白区域。因此这些化合物在抑制包括细胞激活、移动、繁殖和分化的细胞粘着过程中是有用的。这些化合物对抑制、预防和减少VLA-4介导的细胞粘着和与该粘着有关的病状如炎症和免疫反应,包括例如多发性硬化、哮喘、过敏性鼻炎、过敏性结膜炎、炎性肺病、类风湿性关节炎、脓毒性关节炎、I型糖尿病、器官移植、再狭窄、自体骨髓移植、病毒感染的炎性后遗症、心肌炎、包括溃疡性结膜炎和克罗恩氏病的炎性肠病、某些类型的毒性和免疫基肾炎、接触性皮肤过敏症、牛皮癣、瘤转移、多发性骨髓瘤和动脉粥样硬化是有用的。本发明的化合物可以单独使用也可以与抑制、变更、预防或减少细胞粘着的其它治疗或预防性试剂混合使用。本发明还提供了含这些VLA-4-介导的细胞粘着抑制剂的药物制剂和使用本发明的化合物和组合物抑制细胞粘着的方法。
本发明的另一方面涉及本发明的细胞粘着抑制化合物用于制备预防、抑制或减少细胞粘着的药物的用途及其用于制备预防、抑制或减少炎症药物的用途;本发明还涉及细胞粘着抑制化合物用于制备治疗哺乳动物中哮喘、过敏性鼻炎、多发性硬化、动脉粥样硬化、炎性肠病或多发性骨髓瘤的药物的用途;本发明进一步涉及细胞粘着抑制化合物用于制备治疗多发性硬化、炎性肠病以及治疗、预防或改善哮喘症状的药物的用途。
附图简述
图1报道了绵羊用oMePUPA-V处理后的呼吸道反应性。绵羊,天然对猪蛔虫过敏,在以指定剂量给药oMePUPA-V气溶胶或等量载体之后2小时用猪蛔虫过敏原气溶胶攻击。在指定时间测定肺力学并被报道为基于研究前基线值(左方格)的特异性呼吸道阻力的变化。在开始研究之前和过敏原攻击24小时之后(右方格)测定吸入的氨甲酰胆碱的呼吸道阻力。以攻击前和攻击后的PC400(阻力增加400%所需的氨甲酰胆碱的量)值的比报道呼吸道反应性。
图2:绵羊,天性对猪蛔虫过敏,以指定剂量给药oMePUPA-V气溶胶或猪蛔虫气溶胶攻击。测定气溶胶攻击之后的呼吸道阻力的变化并将攻击后峰特异性肺阻力(cm H2O/sec)与基线值比较。与对照组重复比较的Dunnett试验之后,与PBS对照比较,方差单向分析,*=p<0.05。统计显示,与PBS对照组比较的峰特异性肺阻力大大增加。
图3:绵羊,天性对猪蛔虫过敏,在给药oMePUPA-V气溶胶(0.03mg)或等量载体(乙醇∶生理盐水,1∶2,上方格;Tris∶生理盐水,1∶499,下方格)第4天之后用猪蛔虫过敏原气溶胶攻击24小时。在指定时间测定肺力学并被报道为基于研究前基线值(左方格)的特异性呼吸道阻力的变化。在开始研究之前和过敏原攻击24小时之后(右方格)测定吸入的氨甲酰胆碱的呼吸道阻力。以攻击前和攻击后的PC400(阻力增加400%所需的氨甲酰胆碱的量)值的比报道呼吸道反应性。
图4:Balb/c小鼠,先前对DNFB过敏,通过对左耳背面施用DNFB并向右耳背面施用载体攻击。24小时后用微米计测定耳朵的厚度。在用DNFB攻击之后以给定剂量给药oMePUPA-V4小时。以最大有效肠道剂量供给阳性对照(+CTRL)化合物。值为8只动物的平均值±标准误差。上方格显示了耳朵的绝对膨胀。下方格显示了与载体(VEH)对照相比耳朵膨胀抑制的百分比。
图5:在体外通过FACS分析测定α4β1拮抗物的LIBS诱导。在37℃下用仅含2mM MgCl2(Mg+2-TBS)的TRIS缓冲盐水或试验化合物的系列稀释液将Jurkat细胞(2×105/孔)预培养20分钟。将这些样品转移到冰浴中并以10μg/ml的最终浓度补充LIBS抗体9EG7。将这些细胞用Mg+2-TBS冲洗2次并将其再悬浮于在Mg+2-TBS中的1∶200稀释的FITC共轭羊抗大鼠IgG中。通过FACS分析(Becton Dickinson FACScan)测定平均荧光强度(MFI)。上部图显示了用带有1mM Mn+2缓冲液的oMePUPA-V诱导的LIBS。下部图显示了与2mM Mg+2缓冲液相比的oMePUPA-V的LIBS诱导。
本发明提供了能够通过抑制配体结合到受体上抑制VLA-4介导的细胞粘着的化合物。优选的化合物是(R)-N-[[4-[[(2-甲基苯基氨基)羰基]氨基]苯基]乙酰基]-L-脯氨酰基-3-甲基)-β-丙氨酸,本文称之为“oMePUPA-V,”如下式I所示:
oMePUPA-V
并且本文称之为“oMePUPA-V”。本发明还包含oMePUPA-V的药物上可接受的衍生物、盐和酯。
式I的化合物含有一个或多个不对称中心因此可以外消旋混合物、简单的对映体、非对映体混合物和单个非对映体形式存在。本发明包括式I化合物的所有这些异构形式。
本发明还包含药物上可接受的式I盐。术语“药物上可接受的盐”是指由药物上可接受的非毒性碱或酸包括无机或有机碱和无机或有机酸制备的盐。由无机碱获得的盐包括铝、铵、钙、铜、铁、亚铁、锂、镁、锰盐、亚锰、钾、钠、锌等。特别优选铵、钙、镁、钾和钠盐。由药物上可接受的有机非毒性碱获得的盐包括伯、仲和叔胺盐,取代胺包括天然存在的取代胺、环胺和碱性离子交换树脂,如精氨酸、甜菜碱、咖啡因、胆碱、N,N′-二苄基乙二胺、二乙胺、2-二乙氨基乙醇、2-二甲氨基乙醇、乙醇胺、乙二胺、N-乙基-吗啉、N-乙基哌啶、还原葡糖胺、葡糖胺、组氨酸、羟基胺、异丙胺、赖氨酸、甲葡糖胺、吗啉、哌嗪、哌啶、聚胺树脂、普鲁卡因、嘌呤、可可碱、三乙胺、三甲胺、三丙胺、氨丁三醇等。
当本发明的化合物为碱性时,盐可以由包括无机和有机酸的药物上可接受的非毒性酸制备。这些酸包括乙酸、苯磺酸、苯甲酸、樟脑磺酸、柠檬酸、乙磺酸、富马酸、葡萄糖酸、谷氨酸、氢溴酸、盐酸、羟乙磺酸、乳酸、马来酸、苹果酸、杏仁酸、甲磺酸、粘酸、硝酸、扑酸、泛酸、磷酸、琥珀酸、硫酸、酒石酸、对甲苯磺酸等。特别优选柠檬酸、氢溴酸、马来酸、磷酸、硫酸和酒石酸。
此外,本发明包含药物前体,特别是酯前体药物,其中将(R)-N-[[4-[[(2-甲基苯基氨基)羰基]氨基]苯基]乙酰基]-L-脯氨酰基-3-甲基)-β-丙氨酸的羧基用任意醇酯化。优选的醇为甲醇、乙醇、丙醇、丁醇、或直链或支链C1-10烷基醇。
式I化合物对抗VLA-4作用的能力使它们可以用于预防、治疗或逆转由VLA-4结合到其配体上诱导的症状、紊乱或疾病。因此这些对抗剂将抑制包括细胞激活、移动、繁殖和分化的细胞粘着过程。因此,本发明的另一方面提供了治疗、预防、减轻或抑制VLA-4路径所介导的疾病或紊乱。这些疾病和紊乱包括例如哮喘、多发性硬化、过敏性鼻炎、过敏性结膜炎、炎性肺病、类风湿性关节炎、多发性骨髓瘤、脓毒性关节炎、I型糖尿病、器官移植排斥、炎性肠病和其它。
可以使用任意常规技术合成本发明的化合物,在本发明中列举了几种这些技术。优选地,由可容易获得的原料如α-氨基酸及其功能性等价物化学合成这些化合物。合成这些化合物的模块和汇集法也是优选的。在汇集法中,例如在合成的最后阶段,大段最终产物汇聚在一起,而不是通过将小片段增量加成到成长的分子链上。
本发明的化合物还可以通过附加增强选择性生物性能的适宜功能团修饰。这些修饰法在本领域中是已知的并包括增加进入给定生物体系(例如血液、淋巴系统、中枢神经系统)的生物穿透性、增加口服利用度、增加通过注射给药的溶解性、改变新陈代谢和改变排泄速度的那些。这些修饰的例子包括,但不限于,用聚乙二醇的酯化、用新戊酸酯或脂肪酸取代物衍生、转化成氨基甲酸酯、芳环羟基化和芳环中杂原子取代。
本申请全文中所用的术语“患者”是指哺乳动物,包括人。并且术语“细胞”是指任意细胞,优选哺乳动物细胞,包括人细胞。
一旦合成,可以使用体外和体内试验测定本发明化合物的活性和VLA-4特异性。
例如,这些化合物的细胞粘着抑制活性可以通过测定阻断VLA-4-表达细胞结合到纤连蛋白-或CS1-涂布平板上所需的抑制剂的浓度来测定。在这种测定中,微量滴定孔用纤连蛋白(含有CS-1序列)或者用CS-1涂布。如果使用CS-1,它必须共轭到载体蛋白质如牛血清白蛋白上,以便结合到这些孔上。一旦将这些孔涂布,然后将不同浓度的试验化合物与适宜标记的VLA-4-表达细胞一起添加。或者,可以首先添加试验化合物,用所涂布的孔培养,然后加入细胞。使这些细胞在这些孔中培养至少30分钟。培养之后,将这些孔倒空并冲洗。通过定量每种不同浓度的试验化合物和不含试验化合物的对照附着在平板上的荧光性或放射性测定结合抑制。
可以用于本实验的VLA-4-表达细胞包括Ramos细胞、Jurkat细胞、A375黑瘤细胞和人周围血液淋巴细胞(PBL)。可以任意适宜方式,例如荧光或放射性标记,标记本测定中所用的细胞。
还可以使用直接结合测定定量本发明化合物的抑制活性。在该测定中,将含有附着在IgG1分子(“VCAM 2D-IgG”)的铰链区上的首先的两个免疫球蛋白域的VCAM-IgG融合蛋白共轭到标志酶如碱性磷酸酯酶(“AP”)上。该VCAM-IgG融合的合成描述在PCT申请WO90/13300中,将其加入本文作为参考。该熔融与标志酶的共轭是通过本领域中众所周知的交联法完成的。
然后将该VCAM-IgG酶共轭物放入多孔过滤板的孔中,例如在微孔多级筛分测定体系(Millipore Corp.,Bedford,MA)中所含的。然后向这些孔中加入不同浓度的试验抑制化合物,之后加入VLA-4-表达细胞。将这些细胞、化合物和VCAM-IgG酶共轭物混合在一起并在室温下培养。
培养之后,将这些孔抽空,留下细胞和任意附着的VCAM。通过加入与VCAM-IgG共轭的酶的适宜比色底物并测定反应产物的量来确定附着的VCAM的量。反应产物降低说明结合抑制活性增加。下面描述了一些测定方案:
为了评价本发明化合物的VLA-4抑制特异性,测定整联蛋白即β2和β3以及其它β1整联蛋白如VLA-5、VLA-6和α4β7的其它主要基团。这些测定可以与上述的粘着抑制和直接结合测定相似,取代适宜的整联蛋白表达细胞和相应配体。例如,多形核细胞(PMN)在其表面上表达β2整联蛋白并结合到ICAM上。β3整联蛋白涉及血小板聚集作用并且可以在标准血小板聚集测定中测定抑制性。VLA-5特异性地结合到Arg-Gly-Asp序列上,而VLA-6结合到昆布氨酸上。最近发现α4β7为VLA-4同系物,它也结合纤连蛋白和VCAM。在利用上述VCAM-IgG-酶标志共轭物和表达α4β7的细胞系,但不是VLA-4,如RPMI-8866或JY细胞的结合测定中测定α4β7的特异性。
一旦鉴定VLA-4特异性抑制剂,还可以进一步将它们在体内测定中鉴定。一种这样的测定试验在动物中的接触过敏性抑制,例如P.L.Chisholm等人描述的“整联蛋白α-4亚单元的单克隆抗体抑制鼠科接触过敏性反应”,
Bur.J.Immunol.,23,第682-688页(1993)以及“免疫学中的目前方案”中,J.E.Coligan等人编辑,John Wiley & Sons,NewYork,1,第4.2.1-4.2.5页(1991),将它们加入本文作为参考。在该测定中,将动物的皮肤与刺激物如二硝基氟苯接触,然后通过轻微的物理刺激如用尖端轻轻擦涂皮肤使其过敏。恢复一段时间之后,用相同步骤将动物再致敏。过敏几天后,讲动物的一只耳朵与该化学刺激物接触,同时另一只耳朵用没有刺激物的对照溶液处理。将这些耳朵处理之后不久,通过皮下注射给予这些动物不同剂量的VLA-4抑制剂。通过测定处理和未处理的耳朵中动物的耳朵膨胀反应评价与细胞粘着相关的炎症的体内抑制。使用测径规或其它适宜仪器测定耳朵厚度来测定膨胀。以这种方式,人们可以鉴定最适宜抑制炎症的本发明的抑制剂。
用来检测本发明抑制剂的另一体内测定是绵羊哮喘测定。基本上如W.M.Abraham等人在“α4-整联蛋白介导绵羊中抗原诱导的Late Bronchial反应和延长的呼吸道过反应性”,
J.Clin.Invest.,93,第776-87页(1994)中所述的进行该测定,将其加入本文作为参考。该测定测定了过敏绵羊中蛔虫属抗原诱导的后期呼吸道反应和呼吸道过敏反应性的抑制。还可以在血小板聚集测定中检验本发明化合物。
本发明VLA-4抑制剂出人意料地显示出有益的活性和选择性。通常,这些化合物对VLA-4(>1000倍的α4β7和α5β1)具有选择性,在常规PanLabs和非GLP Ames测定中为阴性,在标准辅助药理试验中洁净并在按照人一天一次预定使用量1mg/天或更少在绵羊模型中有效。
与结构上相关的VLA-4抑制剂相比,本发明的化合物具有出人意料优良的效能。例如,蛔虫属过敏的绵羊用雾化药剂以0.1mg/kg一天一次处理4天,然后用抗原攻击24小时,最后剂量之后,预先试验的化合物基本上使早期反应减弱并阻止了后期支气管缩小和非特异性过敏反应性的发展。假设在人中生物等值,那么在70kg人中将需要总剂量7mg。而且,通过气管内管以估计为人口服吸入器装置典型达到的2倍的沉积速度向绵羊给药。此外,可以将赋形剂加入最后固体制剂中,以使装置填充和药物释放最佳。这些因素建议,在人体中超过技术限制1-5mg的14mg或更多的可能剂量需要可以通过干粉吸入器(DPI)装置准确释放。然而所需剂量可以通过该DPI的多次使用释放,这在哮喘市场上将呈现出竞争性缺陷,通常吸入的类固醇计量为0.2-1.0mg。
在抗原攻击之前当以0.003mg/kg的最小剂量以单雾化剂量给药2小时时,oMePUPA-V使早期反应减弱,阻止了后期支气管缩小并使过反应性正常化。而且,以每天剂量0.001mg/kg用抗原攻击4天,最后剂量24小时之后,得到最大反应。因此,与市场上最好的吸入类固醇的剂量水平相比,oMePUPA-V比以前的化合物的效能高出30-100倍。oMePUPA-V及其次末段合成中间物为高度结晶。(参见图1,表1)
此外,与已知VLA-4抑制剂化合物相比,oMePUPA-V具有改善的新陈代谢轮廓。例如,给药气溶胶之后,本发明的化合物很快转变成低活性代谢产物,它是从支气管肺泡流体(BALF)中回收的主要产物,并且也是体循环中观察到的主要产物,在体循环中它比母化合物呈现出更长的血液半衰期。然而向低活性化合物的快速代谢转化是实现减少全身接触的有用的策略,代谢成几乎没有或本质上没有活性的副产物的化合物在进展上呈现出更少的复杂性,并且从后面角度来看是优选的。
由于oMePUPA-V的潜在蛋白水解产物在VLA-4结合测定中无活性,因此蛋白水解将产生无活性产物。尽管如此,体外代谢研究和大鼠、狗和绵羊中的体内PK研究显示出oMePUPA-V在蛋白水解上是稳定的。
表1:与以前已知的抑制剂相比的oMePUPA-V的性能
性能 以前的化合物 oMePUPA-V
抗VLA-4-VCAM-Ig结合的IC50 1.5nM 2.7nM
抗α4β7-VCAM-Ig结合的IC50 2.7μM >100μM
抗α5β1-FN粘着的IC50 >100μM >100μM
绵羊模型中最小有效剂量
-单剂量 0.1mg/kg 0.003mg/kg
-重复剂量 0.03-0.1mg/kg 0.001mg/kg
结晶性 无 有
体外药物筛分85试验 1周击中 干净
ACE活性 ACE底物 干净
葡萄糖醛酸化 低水平 预定的
Ames试验(诱变性) 干净 干净
辅助药理学(副作用) 干净
全身接触,10mg气溶胶剂量(绵羊) 40ng/ml×hr 完成
代谢轮廓 活性新陈代谢产
物
口服利用度 <1% <1%
整体稳定性(40℃,75%RH) “不稳定” 稳定>4周
配制稳定性(40℃) 0.2%降解/天 稳定>4周
可以将本发明的化合物配制成可以经口、非肠道、吸入法喷射、局部、直肠、鼻、口腔、阴道、或通过植入的储器给药的药物组合物。本文中所用的术语“非肠道”包括皮下、静脉内、肌内、关节内、滑膜内、胸骨内、鞘内、肝内、病灶内和颅内注射或输注技术。
本发明的药物组合物含有本发明任意的化合物或其药物上可接受的衍生物和任意药物上可接受的载体。本文中所用的术语“载体”包括可接受的佐剂和载体。可以用于本发明药物组合物的药物上可接受的载体包括,但不限于,离子交换剂、氧化铝、硬脂酸铝、卵磷脂、血清蛋白如人血清蛋白、缓冲物如磷酸盐、甘氨酸、山梨酸、山梨酸钾、饱和植物脂肪酸部分甘油酯混合物、水、盐或电解质如硫酸鱼精蛋白、磷酸氢二钠、磷酸氢二钾、氯化钠、锌盐、胶态的二氧化硅、三硅酸镁、聚乙稀基吡咯烷酮、纤维素基物质、聚乙二醇、羧甲基纤维素钠、聚丙烯酸酯、蜡、聚乙烯-聚氧丙烯-嵌段聚合物、聚乙二醇和羊毛脂。
根据本发明,药物组合物可以为可无菌注射制剂的形式,例如可无菌注射的含水或含油悬浮液形式。可以使用适宜的分散或润湿剂和悬浮剂根据本领域中已知的技术配制该悬浮液。可无菌注射的该制剂还可以为非毒性非肠道可接受的稀释剂或溶剂中的可无菌注射的溶液或悬浮液,例如在1,3-丁二醇中的溶液。可以接受的载体和可以使用的溶剂为水、林格溶液和等渗氯化钠溶液。此外,无菌固定油常用作溶剂或悬浮介质。为此目的,可以使用包括合成的单或二甘油酯的任意混合不挥发油。脂肪酸,例如油酸和其甘油酯衍生物以及作为天然药物上可接受的油,如橄榄油或蓖麻子油,特别是它们的聚氧乙基化变体在制备可注射物中是有用的。这些油溶液或悬浮液还可以含有长链醇稀释剂或分散剂。
本发明的药物组合物可以任意口服可接受的剂量形式口服给药,这些形式包括,但不限于,胶囊、片剂、含水悬浮液或溶液。在为口服用的片剂时,常用的载体包括乳糖和玉米淀粉。典型地还加入如硬脂酸镁的润滑剂。对于以胶囊形式口服而言,有用的稀释剂包括乳糖和干玉米淀粉。当口服用需要含水悬浮液时,将该活性组分与乳化和悬浮试剂混合,如果需要的话,还可以添加某些甜味剂、调味剂或着色剂。
另外,本发明的药物组合物可以直肠投药的栓剂形式给药。可以通过将该试剂与适宜的在室温下为固体但在直肠温度下为液体并因此熔于直肠中释放该药物的无刺激赋形剂混合来制备它们。这些物质包括可可脂、蜂蜡和聚乙二醇。
还可以经局部给药本发明的药物组合物,特别是当所处理的靶子包括通过局部涂敷可以容易地达到的区域或器官,包括例如眼、皮肤或下面肠道的疾病。对于每种这些区域或器官,能够容易地制备适宜的局部制剂。
可以直肠栓剂(参见上面的)或适宜的灌肠剂实现下面肠道的局部施加。还可以使用局部透皮贴剂。
为了局部施加,可以将药物组合物配制成含悬浮或溶解于一种或多种载体中的活性组分的适宜软膏。局部给药本发明组合物的载体包括,但不限于,矿物油、液体凡士林、白色凡士林、丙二醇、聚氧乙烯、聚氧丙烯化合物、乳化石蜡和水。或者,可以将该药物组合物配制成含有悬浮或溶于一种或多种药物上可接受的载体中的该活性组分的适宜洗液或乳膏。适宜的载体包括,但不限于,矿物油、脱水山梨糖醇单硬脂酸酯、吐温60、鲸蜡基酯石蜡、鲸蜡醇、2-辛基十二烷醇、苯甲醇和水。
对眼用而言,可以将该药物组合物配制成在等渗、pH经过调整的无菌生理盐水中的微粒化悬浮液,或者优选在有或没有例如氯化苯甲羟胺的等渗、pH经过调整的无菌生理盐水中的溶液。或者,对眼用而言,可以将该药物组合物配制在例如凡士林的软膏中。
还可以通过鼻气溶胶或通过使用雾化器、干粉吸入器或计量吸入器吸入给药本发明的药物组合物。根据药物制剂领域中众所周知的技术制备这些组合物并可使用苯甲醇或其它适宜的防腐剂、提高生物利用度的吸收促进剂和/或其它传统增溶或分散剂将它们制成生理盐水的溶液。此外,本发明的组合物可以包括任意药物上可接受的载体,例如用于干粉制剂的乳糖。
可以与载体材料混合生产单剂量形式的活性组分的量随所处理的宿主和给药的具体方式而变化。但是,应理解为,任意特定患者的具体剂量和处理机制将取决于很多因素,包括具体所用化合物的活性、年龄、体重、一般健康状况、性别、饮食、给药时间、排泄速度、药物组成和处理医师的判断和所处理的特定疾病的严重性。活性组分的量还可能取决于治疗或预防试剂,如果有的话,将其与该组分共同给药。
对预防、减轻或抑制细胞粘着有效的本发明组合物的剂量和给药速度将取决于很多因素,如抑制剂的性质、患者大小、处理的目标、待处理的病状的性质、所用的特定药物组合物和处理医师的判断。每天每kg体重约0.001-约100mg、优选约0.01-约50mg并且更优选约10mg的该活性组分化合物的剂量水平是有用的。
就使用静脉内给药的组合物而言,适宜剂量范围为约0.001mg-约25mg/kg、更优选约0.01mg-约1mg/kg。
根据另一实施方式,含有本发明化合物的组合物还可以含有第二种试剂,它们选自皮质类固醇、支气管扩张药、平喘药、肥大细胞稳定剂、消炎药、抗风湿剂、免疫抑制剂、抗代谢物、免疫调制剂、治牛皮癣药和治疗糖尿病药。每种这些类的特定化合物可以选自下面适宜组标题所列的任意那些:“综合性药用化学品”英国牛津Pergamon出版社,第970-986页(1990),将其内容引入本文作为参考。在该组中还包括了如下化合物:茶叶碱、柳氮磺胺吡啶、对氨基水杨酸盐(消炎药);环孢菌素、FK-506和雷帕霉素(免疫抑制剂);环磷酰胺和甲氨蝶呤(抗代谢物);类固醇(吸入、口服或局部)和干扰素(免疫调制剂)。而且,可以将本发明的化合物与其它细胞粘着抑制剂一起给药。当与所述VLA-4抑制剂一起给药一种或多种其它试剂时,可以将这些活性组分配在一起,或者可以结合给药。基本上可以同时或依次给药与本发明的VLA-4抑制剂结合的一种或多种活性试剂。根据所给予的试剂、所需结果和处理的患者及其条件,本领域技术人员可以容易地测定最适宜的给药。
根据其它实施方式,本发明提供了预防、抑制或减轻患者中与细胞粘着相关的炎症和与细胞粘着相关的免疫或自体免疫反应的方法。与VLA-4-相关的细胞粘着在许多炎症、免疫和自体免疫疾病中起核心作用。因此,可以将通过本发明化合物的细胞粘着抑制剂用于治疗或预防炎症、免疫和自体免疫疾病的方法中。优选用本发明方法治疗的疾病选自哮喘、关节炎、牛皮癣、移植排斥、多发性硬化、糖尿病和炎性肠病。
这些方法可以在单疗法中使用本发明的化合物或者与消炎药或免疫抑制剂结合使用。这些结合疗法包括以单剂量形式给药试剂或以复合剂量形式同时或不同时间给药。
实施例
实施例1:
oMePUPA-V的制备
oMePUPA-V,(R)-N-[[4-[[(2-甲基苯基氨基)羰基]氨基]苯基]乙酰基]-L-脯氨酰基-3-甲基)-β-丙氨酸,是在汇集合成中由商购的琥珀酰亚氨基Boc-(L)-脯氨酸(Boc-Pro-OSu;Bachem)和(R)-苯甲基-3-氨基丁酸半硫酸盐(Celgene Corp.)制备的。原料在有Et3N下在CH2Cl2中偶合,然后用二噁烷中的4N HCl水解Boc基团,从CH2Cl2/Et3O中重结晶,得到HCl盐。将该HCl盐与用相应酸MPUPA-OH(Ricerca,Inc.)制备的琥珀酰亚氨基-2-[4-[2-(甲基苯基氨基羰基)]氨基苯基乙酸酯(盐)(MPUPA-OSu)偶合,提供结晶oMePUPA-V-苯甲酯,将其在THF/H2O(9∶1)中催化氢化(10%Pd/C)得到oMePUPA-V。在从20%含水丙酮中重结晶之后,获得的最终产物为白色固体。
理化特性汇总
化学名称:(R)-N-[[4-[[(2-甲基苯基氨基)羰基]氨基]
苯基]乙酰基]-L-脯氨酰基-3-甲基)-β-丙氨
酸
分子式: C25H30N4O5
分子量: 466.53
外观:洁净白色粉末
熔点:153.6-154.4℃
方案1:
由MPUPA-OH(1)制备MPUPA-OSu(2)
方案2:
由Boc-(L)-Pro-OSu(3)和苯甲基-(R)-3-氨基丁酸半硫酸酯(盐)(4)
用于制备oMePUPA-V的合成化学描述在方案1和2中。由商业源和合同厂商获得这些原料:由Ricerca,Inc.,Painesville,OH大量制备(1);从Bachem Bioscience,Inc.,King of Prussia,PA获得(3)并从CelgeneCorp.,Warren,NJ获得(4)。
oMePUPA-V的制备:
常规化学方法(1H NMR,13C NMR.MS,IR & HPLC)
在Bruker AC 300或Varian 500或Varian 600仪器上进行1H NMR测定,或者在DMSO-d6中并参照DMSO-d6(d 2.49ppm)或者在CDCl3中并参照残余CHCl3(d 7.24ppm)测定样品。
在Varian 500或Varian 600仪器上进行13C NMR测定,或者在DMSO-d6中并参照DMSO-d6(d 40.5ppm)或者在CDCl3中并参照CDCl3(d 77.0ppm)测定样品。
在带有HP 1500型自动取样器的Fisons VG Platform LC-MS-DS质谱仪体系上进行质谱分析,并使用Fisons VG MassLynx质谱仪工作站处理数据。在VG Analytical ZAB 2SE高场质谱仪上使用快速原子轰击以M型扫描(PA)进行该HRMS工作,参照SOP#MS-002,MS-006,MS-012和MS-023。使用铯离子枪产生所需质谱的离子,它是使用PDP-11-250J数据体系记录的。
在Perkin Elmer 1600系列FTIR上进行IR谱测定。
分析HPLC色谱法按如下进行:
1.使用带PB Nelson 3020积分仪的Perkin Elmer 785A UV检测器(固定在214nm)和应用生物体系783A UV检测器(固定在254nm)的PerkinElmer 200系列HPLC自动取样器体系获得使用程序1(Equilibrate@20%B,注射样品,20%B(1分钟),20%-70%B(24分钟),70%-100%B(17分钟))的色谱图。仅报道了面积百分比值。
2.使用带783A波长UV检测器的应用生物体系400溶剂释放体系和Waters717自动取样器获得使用程序8(Equilibrate@15%B,注射样品,15%B(1分钟),15%-40%B(25分钟),40%B(10分钟))的色谱图。使用HP 3396系列II积分仪处理该数据。用以下参数调整积分仪:衰减=8,阈值=5,注射面积=10000,峰宽=0.04,记录纸速=0.2。使用Vydac C-18柱(5m孔径,4.5mm×25cm,测试#218TP54)进行所有HPLC工作。
溶剂A(水+0.1%TFA)
溶剂B(乙腈+0.1%TFA)
流速=1mL/分钟
梯度程序如下:
程序1:Equilibrate@20%B,注射样品,20%B(2分钟),20%-70%B(25分钟),100%B(5分钟)。
[4-[[[(2-甲基苯基)氨基]羰基]氨基]苯基]乙酸的理化数据(1,
MPUPA-OH;由Ricerca Inc.生产的材料):
mp 210-215℃(分解);
IR(KBr)3295(宽带),3034(宽带),1107,1637,1603,1551,1516,1457,1414.1302,1241,1189,1118cm-1;
1H NMR(600MHz,DMSO-d6)d12.28(bs,1H),9.0(s.1H),7.91(s,1H),7.88(d.J=7.8Hz,1H),7.43(d,J=8.4Hz,2H),7.19(d,J=8.4Hz,2H),7.16(m.2H),6.94(dd,J=7.8,8.4Hz,1H),3.51(s,2H),2.25(s,3H);
13C NMR(150MHz.DMSO-d6)d173.0(C),152.7(C),138.5(C),137.5(C),130.2(CH),129.8(CH),128.3(CH),127.5(CH),126.2(CH).122.7(CH),121.0(CH),118.1(CH),40.1(CH2),179(CH3);
MS(EI)m/z 285(M+1)+,193,152,134,132,109,108,106,93,91,57;
C16H16N2O3的元素分析,理论值:C,67.59;H,5.67;N,9.85;实测值:C,67.60;H,5.70;N,10.01。
琥珀酰亚氨基[4-[[[(2-甲基苯基)氨基]羰基]氨基]苯基]乙酸酯的
制备(2,MPUPA-OSu)
在10分钟内边剧烈搅拌边向在乙腈(600rnL)中的o-甲基苯脲苯乙酸(1,MPUPA-OH;150g,0.501mol;来自Ricerca,Inc.)回流悬浮液中加入亚硫酰氯(41mL,0.558mol)。离析出大量HCl。继续搅拌1.5小时并将反应混合物冷却到室温。该反应混合物转变成粉红色浆液,向其中加入一部分固体N-羟基琥珀酰亚胺(HOSu;75.5g,0.636mol)。在30分钟内向该混合物中滴加三乙胺(174rnL),同时用水浴将反应混合物的温度保持在60℃以下。继续搅拌2小时,然后向该反应混合物中加入蒸馏水(500mL)。过滤出固体并用2L蒸馏水和乙腈(2×200mL)冲洗,空气干燥,在真空(-0.1mmHg)下在P2O5中进一步干燥,得到淡棕色粉末粗产物(175g,97%产率)。粗产物(174g)从乙腈(3.5L)中重结晶并用活性炭(10g)脱色,得到129g白色MPUPA-OSu粉末(2;68%产率)(纯度>99%)。mp 211.2-211.8℃;
IR(KBr):3905-3203(宽带),1816,1783,1654,1368,1304,1244,1116,1021cm-1;
1H NMR(300MHz,DMSO-d6):d9.04(s.1H).7.92(s.1H),7.82(d,1H),7.44(d,J=8.5Hz,2H),7.24(d,J=8.5Hz,2H),7.15(m,2H),6.93(dd,J=7.4,7.3Hz,1H),4.02(s,2H),2.80(s,4H).2.23(s,3H);
MS(EI.ES+)rn/z 382[(M+1)+],239,108,106。
琥珀酰亚氨基Boc-(L)-脯氨酸(Boc-Pro-OSu,3;从Bachem
Bioscience获得的材料)的理化数据:
mp 132-136℃;
IR(KBr)3456,2940,1731,1619,1561,1541,1497,1454,1395,1337,1259,1202,1118,1060cm-1;
1H NMR(300MHz,CDCl3)d4.51(dd,J=3.8,8.7Hz,1H),3.56(m,1H),3.44(m,1H),2.80(s.4H),2.32(m,1H),2.27(rn,1H),1.94(m.2H),1.43(s,9H);
MS(EI)m/z 335(M+N2)+,279,213,138,114,86;
HPLC 97.1%。
苯甲基-(R)-3-氨基丁酸半硫酸酯(4;从Celgene Corp.获得的材料)
的理化数据:
mp 249.4-249.8℃;
IR(KBr)3515,3383,2989,2945,2880,1821,1788,1744,1701,1476,1454,1421,I394,1368,1260,1241,1202,1159,1077crn-1;
1H NMR(300MHz,CDCl3)d7.85(bs,2H),7.26(s,5H),5.06(ABq,J=12.3Hz.2H),4.35(m,2H),3.73(m.1H),2.92(dd,J=6.4,17.1Hz,1H),2.66(dd,J=6.4,17.0Hz,1H),1.35(d,J=6.5Hz,3H);
MS(EI)m/z 195(M+3)+,194(M+2)+,106,92,91;
HPLC 99.0%.
N-(叔丁氧羰基)-L-脯氨酰-3-甲基-(R)-β-丙氨酸苯甲基酯(5)的制
备
向CH2Cl2(200mL)中的苯甲基-R-3-氨基丁酸半硫酸酯(盐)(4;66.7g,213mmol)的充分搅拌悬浮液中加入Boc-(L)-Pro-OSu(3;53.9g,222mmol)和Et3N(95mL,681mmol)。在室温下将该反应混合物搅拌2小时。将该反应混合物在EtOAc(1.5L)和H2O(250mL)之间分开,有机层用10%柠檬酸(3×250mL)、H2O(250mL)、饱和碳酸氢钠(250mL)、H2O(250mL)和生理盐水(3×250mL)洗涤,经Na2SO4干燥并在旋转蒸发器(40℃;-80mmHg)上经第一次浓缩,然后在高真空(室温,16小时;0.2mmHg)下浓缩,得到粘性油中间体5(88.1g),它含残余EtOAc和CH2Cl2(通过NMR)且其纯度>98%(HPLC)。该材料不用进一步提纯下就可用于下面反应。
1H NMR(300MHz,CDCl3)d7.30(m,5H),6.44(bs,1H),5.10(dd,J=12.3,14.1Hz,2H),4.32(m,1H),4.13(m,1H),3.34(bs,2H),2.48(d,J=5.1Hz,2H),2.1(m,2H),1.75(bs,2H),1.40(s.9H),1.17(d,J=6.0Hz,3H);
MS(EI):m/z 413[M+Na]+,313,291,191,194,165,91。
L-脯氨酰基-3-甲基-(R)-β-丙氨酸苯甲基酯盐酸盐(6)的制备
向来自上面反应的中间体5中慢慢加入在二噁烷(240mL)中的4N HCl溶液。保证快速放出气体(小心:放热)。将该反应混合物搅拌2小时,然后在旋转蒸发器(45℃;-80mmhg)上经第一次浓缩,然后在高真空(室温,14小时;0.2mmHg)下浓缩一夜,得到极粘材料,将其从CH2Cl2/Et2O(600mL/700mL)中结晶,得到64.0g(92%两步的总产率)白色固体HCl盐6(HPLC纯度99.6%)。
mp 119.8-120.5℃;
IR(KBr):3217,3072,2904,2756,1736,1681,1560,1446,1387,1352,1295,1244,1178,1096crn-1;
1H NMR(500MHz1 CDCl3)d10.21(bs.1H),8.71(d,J=8.0Hz,1H),7.77(bs,1H),7.24(m.5H).5.00(s.2H),4.52(bs.1H),4.22(表观t,J=6.5Hz.1H),3.33(bs,2H),2.67(dd,J=5.5,15.5Hz,1H),2.44(m,2H),1.89(m,3H),1.15(d,J=6.5Hz,3H);
13C NMR(125MHz,CDCl3)d171.03(C=O),167.67(C=O).135.58(C),128.43(CH),128.13(CH),128.06(CH),66.34(CH2),59.71(CH),46.55(CR2),43.34(CH),40.42(CH2),30.50(CH2),24.23(CH2),19.92(CH3);
MS(EI)m/z 291[M-Cl]+,199,194,160,139,92,91;
C16H23N2O3Cl的元素分析、计算:C,58.80;H,7.094;N,8.57;实测:C,58.95;H,6.99;N,8.46.
N-[[4-[[(2-甲基苯氨基)羰基]氨基]苯基]乙酰基]-L-脯氨酰基-3-
甲基)-(R)-β-丙氨酸苯甲基酯(7)的制备
向DMF(125mL)中的HCl盐6(61.77g,189mmol)溶液中加入MPUFA-OSu(2;69.39g,181.9mmol),然后加入Et3N(90mL;pH 10)。将该反应混合物搅拌3.5小时,然后用EtOAc(1L)稀释并用H2O(3×250mL)提取。这时产物开始沉淀。将10%柠檬酸溶液(250mL)添加到有机层中(小心:放热!),摇动,形成很多沉淀。在多孔玻璃漏斗(2L,M)上过滤该固体。将该固体用柠檬酸(10%,2×250rnL)、H2O(250mL)、饱和碳酸氢钠(2×250mL),H2O(250mL)和生理盐水(3×250mL)洗涤,在该漏斗上通过抽吸(-80mmHg)将其干燥1夜(-14小时),得到黄白色固体,将其从THF/Et2O(1L/4L)中重结晶,得到83.3g白色固体化合物7(HPLC纯度99.6%)。
将滤液进一步用柠檬酸(10%,3×250ml)、H2O(250mL)、饱和碳酸氢钠(2×250mL)、H2O(250mL)和生理盐水(3×250rnL)洗涤。伴随每次含水洗涤,其他化合物沉淀出来;但是继续洗涤,小心别使沉淀物损失。过滤,得到4.02g白色固体产物。最后将该滤液用Et2O(1L)稀释,过滤,固体用Et2O(3×100mL)洗涤,得到1.67g主白色固体的另一收获物。该反应的总产率为88%。
mp 153-153.5℃;
IR(KBr)3342,3307,3119,2966,1737,1702,1643,1590,1543,1514,1455,1414,1308,1238,1179crn-1;
1H NMR(500MHz,DMSO-d6):a3:2旋转异构体混合物,(主构象峰):d9.00(bs,1H),7.91(bs,1H),7.84(d,J=8.3Hz,1H),7.68(d,J=8.3Hz,1H),7.40-7.28(m,7H),7.13(3H),7.06(d,J=8.8Hz,1H),6.92(t,J=7.3Hz.1H),5.06(ABq,J=12.2Hz,Dn=8.9Hz,2H),4.18(dd,J=3.4,8.8Hz.1H),4.10(四重峰,J=6.8Hz,1H).3.57(m,2H),3.50-3.22(m,3H).2.62-2.37(m,2H),2.23(s,3H),2.18-1.68(rn,3H),1.05(d,J=6.8Hz,3H)和(次构象峰):d9.00(bs.1H),7.91(bs,IH),7.84(d,J=8.3Hz,1H),8.15(d,J=8.3Hz,1H),7.40-7.28(m,7H),7.13(3H),7.06(d,J=8.8Hz,1H),6.92(t,J=7.3Hz,1H),5.01(ABq,J=12.2Hz,Dn=19.0Hz.2H),4.32(dd.J=2.4,8.8Hz,1H),4.22(四重峰,J=6.8Hz,1H).3.57Cm,2H),3.50-3.22(m,3H),2.62-2.37(m,2H),2.23(s,3H),2.18-1.68(m,3H),1.10(d,J=6.8Hz,3H);
13C NMR(125MHz,DMSO-d6):旋转异构体混合物,(主构象峰):d170.80(C=O),170.52(C=O),169.18(C=O),152.61(C=O),138.10(C),137.38(C),136.04(C),130.05(CR),129.63(CH),129.47(CH),128.5S(C),128.28(CH),127.89(CH),127.85(C),126.02(CH),122.50(CH),117.90(CH),117.81(CH),65.44(CH2),59.61(CH),47.04(CR2),41.75(CH),40.41(CH2),40.00(CH2),29.29(CH2),24.13(CH2),19.88(CH3),17.78(CH3)和(次构象峰):d170.94(C=O),170.52(C=O),169.31(C=O),152.61(C=O),138.10(C),137.38(C),136.04(C),130.05(CH),129.63(CH),129.47(CH),128.65(C),128.28(CH),127.89(CH),127.85(C),126.02(CH),120.940(CH),117.90(CH),117.81(CH),65.44(CH2),59.91(CH),46.51(CH2),42.01(CH),40.13(CH2),39.84(CH2),31.75(CH2).22.11(CH2),20.05(CH3),17.78(CH3);
MS(EI):m/z 579[M+Na]+,557,454,426,357,336,293,267,201;
C32H36N4O5的元素分析、计算:C,69.05;H,6.52;N,10.07;实测:C,68.87;H.6.52;N,9.93.
N-[[4-[[(2-甲基苯基氨基)羰基]氨基]苯基]乙酰基]-L-脯氨酰基
-3-甲基)-(R)-β-丙氨酸(8:oMePUPA-V)的制备
在有Pd/C(10%;2.44g)的情况下在-55psi下将THF/H2O(9∶1;800rnL)中的OMePUPA-V-OBn(7;80.18g)溶液氢化。25小时后,将反应混合物通过多孔玻璃漏斗上的Solka Floc(144g;Fiber Sales & DevelopmentCorp.)过滤。然后将滤液通过另一块Solka Floc(115g)再过滤,浓缩至约250mL,慢慢倒入剧烈搅拌的甲苯(3L)中。将悬浮液搅拌0.5小时,过滤(2L多孔玻璃漏斗),将所得白色粉末首先在漏斗上通过抽吸(约80mmHg;0.5小时)然后在真空炉(14小时;45℃,用N2流将压力调整到25inHg真空度)干燥。将该白色节块粉碎(研钵和研棒)成细粉,得到58.3g(产率87%)的oMePUPA-V白色固体。将该产物从丙酮/H2O(320mL/75mL)中重结晶。将晶体收集并首先在多孔玻璃漏斗上通过抽吸(1小时,80mmHg)然后在真空炉(25小时;45℃;通过N2流将压力调整到25inHg真空度)中干燥,得到47.0g(84%,通过重结晶回收)oMePUPA-V白色固体(HPLC纯度99.1%)
mp 153.6-154.4℃;
IR(KBr)3354,3307,1719,1643,1590,1543,1514,1449,1414,1308,1237cm-1;
1H NMR(600MHz,DMSO-d6):3:2旋转异构体混合物(主构象峰):δ12.21(bs,1H),8.99(s,1H),7.91(s,1H),7.87(d,J=8.2Hz,1H),7.68(d,J=7.9Hz,1H),7.40(d,J=8.6Hz,2H),7.17(d,J=5.9Hz,2H),7.15(d,J=7.7Hz,1H),7.12(dd,J=7.9,8.2Hz.1H),6.94(dd.J=7.3,7.3Hz,1H),4.22(dd,J=3.3,8.8Hz,1H),4.06(m,J=6.6Hz,1H).3.47(dd,1H),3.44(d,J=15.0Hz,1H),3.37(dd,1H),3.29(d,J=15.4Hz,1H),2.46(dd,1H),2.27(m.1H),2.25(s,3H),1.99(rn,1H),1.80m(rn,1H),1.78(m,1H),1.76(m,1H),1.07(d,J=6.6Hz,3H)和(次构象峰):δ12.21(bs,1H).8.99(s,1H).7.90(s,1H),7.87(d,J=8.2Hz,1H),8.12(d,J=8.2Hz,1H),7.40(d,J=8.6Hz.2H),7.16(d,J=5.9 Hz.2H),7.15(d,J=7.6Hz,1H),7.12(dd,J=7.9,8.2Hz,1H),6.94(dd,J=7.3,7.3Hz,1H),4.34(dd,J=1.8,8.4Hz,1H),4.18(m,J=6.6Hz,1H),3.60(m,2H),3.59(m,1H),3.48(m.1H).2.47(dd,J=6.6,15.4Hz,1H),2.40(dd,J=6.6,15.4Hz.1H),2.25(s.3H),2.15(m.1H),1.83(rn,1H),1.91Cm.1H),1.77(m,1H),1.12(d,J=6.6Hz,3H);
13C NMR(150MHz.DMSO-d6)(主构象峰):δ172.4(C=O),170.9(C=O),169.3(C=O),152.6(C=O),138.2(C),137.5(C),130.2(CH),129.8(CH),129.6(CH),128.7(C),127.4(C),126.1(CH),122.6(CH),120.9(CH),118.0(CH),117.9(CH),59.7(CH),46.6(CH2),41.7(CH2),40.6(CH2),40.2(CH2),29.4(CH2),22.2(CR2),19.9(CH3),17.9(CH3)和(次构象峰):δ172.5(C=O),171.0(C=O),160.5(C=O),152.7(C=O),138.19(C),137.5(C),130.2(CH),129.8(CH),129.6(CH),128.8(C),127.4(C),126.1(CH),122.6(CH),120.9(CH),118.0(CH),117.9(CH),59.9(CH),47.1(CH2),42.0(CH2),39.8(CH2),40.3(CH2),31.8(CH2),24.2(CH2),20.2(CH3),17.9(CH3);
MS(EI)rn/z 468[M+H]+,336,267,137;
C25H30N4O5的元素分析、计算:C,64.36;H,6.48;N,12.61;实测:C,64.07;H,6.40;N,11.85。
实施例2.
在过敏性肺炎的绵羊模型中的活性
使用重量在27-50kg之间的过敏性绵羊。所有绵羊已提前显示出对吸入的雾化猪蛔虫过敏原产生早期和晚期的支气管反应。这些绵羊是清醒的并将它们以伏卧位绑在经过改装的运货马车中使它们的头不能移动。通过2%利多卡因将其鼻表面麻醉,首先将球形导管通过鼻孔进入下食道。使用柔性光学纤维支气管镜作为导向装置通过另一鼻孔将成套气管内管插入这些动物内。本研究中所用的所有方案都是得到Mount SinaiMedical Center Animal Research Committee许可的,它对保证试验动物的人道护理和使用负责。使用食管的球状导管(填充有1mL空气)评价胸膜压力,该导管位于离胃食管接合处5-10cm。在该位置,末端呼气胸膜压范围为-2至-5cmH2O。一旦放置该气球,就保证了它在实验过程中保持在相同位置。用通过并位于气管内管顶端远端的侧孔导管(内径,2.5mm)测定气管内的侧压。
将气管和胸膜压力导管连接到不同压力传感器(MP45,Validyne,Northridge,CA),用于测定定义为气管和胸膜之间压差的跨肺压。通过将气管内管的邻近端与呼吸速度描记器(Fleisch,Dyna Sciences,Inc.,Blue Bell,PA)相连测定气流。在与80-386 DOC个人计算机相连的多波道生理记录器上记录跨肺压和流动信号,以联机计算跨肺压的变化除以中潮体积流动的变化(通过数位积分获得)的平均肺流阻(RL)。将至少5次没有人为吞咽现象的呼吸的平均值用于获得RL(以cmH2O/L/sec计)。测定RL之后即刻在恒定体积壳体体积描记器中测定胸的气体体积(Vtg),从而获得特异性肺阻力(specific lung resistance)(SRL=RLxVtg)(以LxcmH2O/L/sec计)。
使用一次性药用空气喷射雾化器(Raindrop,Puritan Bennett,Lenexa,KS)产生所有液体剂量气溶胶,该雾化器赋予气溶胶3.2μm的质量平均空气动力直径(由Andersen阶式碰撞取样器测定)。该雾化器与放射剂量计体系相连,该体系由电磁阀和压缩气源(20psi)组成。将雾化器出口导入塑料T接头,该接头一端与活塞呼吸罩(Harvard Apparatus,S.Natick,MA)的吸气端口相连。在开始呼吸罩吸气循环时将该电磁阀打开一半。以500mL的潮流气量和20次/分钟的呼吸速度输送气溶胶。为了评价支气管反应性,通过吸入缓冲剂后即刻和每次连续给药10次呼吸递增浓度的卡巴胆碱(以0.25、0.5、1.0、2.0和4.0%w/v于缓冲生理盐水中)之后测定SRL来完成卡巴胆碱的累积浓度反应曲线。当SRL增加超过给予生理盐水后的值400%或在给予最高卡巴胆碱浓度之后停止该激发试验。通过测定SRL增加到由剂量反应曲线内推的给予生理盐水后的值的400%(PC400)的累积卡巴胆碱浓度(以呼吸单位计)评价支气管反应性。1呼吸单位(BU)定义为一次呼吸1%w/v卡巴胆碱雾化溶液。
将oMePUPA-V剂量溶于1∶2乙醇:生理盐水、1∶5乙醇:200mM磷酸钠或Tris缓冲剂中。当使用Tris时,使用生理盐水进行任意所需稀释。以总体积3-5mL制备剂量。
在所有研究中,在开始研究之前3-4天测定基线呼吸道反应性(即PC400)。在单剂量预处理研究中,测定SRL并用该化合物或载体处理动物。在处理后2小时(就在攻击之前)再测定SRL,然后用过敏原攻击动物。在多剂量研究中,在过敏原攻击之前头4天,一天一次对动物处理4天并在最后剂量之后24小时用过敏原攻击。在化合物最后剂量或载体处理之前或之后测定SRL。在所有研究中,在过敏原攻击之后即刻、攻击后1-6小时每小时、过敏原攻击后6.5-8小时中每半小时再测定SRL。在过敏原攻击后24小时进行呼吸道反应性的后攻击测定(PC400)。
值以平均值±平均值的标准误差来表示。以与攻击前的基线SRL的差计算每只绵羊的SRL的变化。攻击后SRL的变化以早期呼吸道反应(EAR)来表征,该反应约进行0-4小时。接着进行后期呼吸道反应(LAR),该反应在过敏原攻击之后约4-8小时进行。使用梯形规则计算每个动物的EAR和LAR曲线的面积。与安慰剂对照相比该EAR或LAR曲线面积的大大降低显示出对过敏原诱导的SRL变化的治疗效果。在过敏原攻击之前和攻击之后24小时时评价的卡巴胆碱的呼吸道反应性(PC400)是以每只绵羊的PC400比(攻击前/攻击后的PC400值)表示的。与安慰剂对照相比,该PC400比大大增加,说明有治疗效果。使用遵循与对照的多重对比的Dunnett试验的单向方差分析(单尾)进行与安慰剂对照的对比。产生p<0.05的比较呈现出统计学上是有效的。
图1显示了给药2小时后在对猪蛔虫过敏的绵羊中气溶胶化oMePUPA-V的抑制剂量反应。左方格显示了特异性肺阻力SRL(以cm H2O/sec计)的变化。右方格显示了攻击后24小时测定对吸入的卡巴胆碱的呼吸道反应性(PC400比,攻击前/攻击后)。oMePUPA-V以剂量0.01-0.03mg不能抑制早期或后期呼吸道反应或改变过敏原攻击后24小时对卡巴胆碱的过反应性。剂量0.1、1和3抑制早期呼吸道反应并最大地抑制后期呼吸道反应。这些剂量还抑制过敏原攻击后24小时对卡巴胆碱的过反应性。将这些数据的统计分析示于表2中。
表2
| 处理 | 剂量(mg) | 载体 | n | EAR(ΔSLR x h) | LAR(ΔSLR x h) | PC400(后/前) |
| 在过敏原攻击之前2小时给药 | ||||||
| PBSoMePUPA-V | 0.010.03 | EtOH:NSEtOH:NS | 1222 | 5.85±0.626.87±0.0510.62±3.91 | 4.85±0.695.11±1.463.98±0.23 | 0.49±0.030.44±0.040.43±0.00 |
| 0.101.003.00 | EtOH:NSEtOH:PBSEtOH:PBS | 422 | 2.54±0.74*2.14±0.702.47±0.62 | 0.67±0.17*0.27±0.34*0.68±0.07* | 1.18±0.11*1.05±0.11*1.07±0.08* |
绵羊,天性对猪蛔虫过敏,在以指定剂量给予oMePUPA-V气溶胶或等量载体之后2小时或者重复每天给药阈下剂量oMePUPA-V或等量BPS4天后24小时用猪蛔虫过敏原气溶胶攻击。肺力学,基于研究前基线值的特异性呼吸道阻力的变化报道,在过敏原攻击后测定了8个小时。早期呼吸道反应(0-4小时,EAR)和后期呼吸道反应(4-8小时,LAR)以Δ特异性肺阻力曲线x时间的平均面积±标准误差表示。在研究开始之前和过敏原攻击后24小时测定对吸入的卡巴胆碱的呼吸道阻力。呼吸道反应性以攻击前和攻击后的PC400值(阻力增加到400%所需的卡巴胆碱的量)之比报道。
根据与对照组的多重比较的Dunnett试验,与PBS对照相比,单向方差分析*=p<0.05。这显示经统计EAR或LAR大大降低,或者与PBS对照组相比PC400比大大增加。
单剂量刺激
在用猪蛔虫过敏原攻击之后,通过与基线阻力相比的呼吸道阻力没有变化反映出,上面研究中所用的oMePUPA-V剂量没有一种具有刺激效果。这显示在图2中。
重复剂量研究
图3描述了当以单剂量用于急性预处理时显示无效的0.03mg剂量的oMePUPA-V,如果一天一次给药4天,当在最后剂量后24小时给以抗原攻击时,却有保护性。上下左手方格显示出,使用两种不同配方可以看出这种效果。由图3的上下右手方格可以看出,在另外24小时后对卡巴胆碱的过敏反应性还被最大抑制。oMePUPA-V抗EAR和LAR及抗对卡巴胆碱的过反应性的这种保护性效果很大,这种定量分析显示在表3中。
该研究的结果说明,通过气溶胶用小分子抑制剂VLA-4、oMePUPA-V的单个预处理能够预防过敏绵羊模型中过敏原诱导的早期和后期呼吸道反应和后过敏原诱导的AHR。以单个预处理,用任意剂量oMePUPA-V看不出呼吸道的刺激效果。结果还显示出,用多次处理可以降低oMePUPA-V的有效剂量。这些数据共同地提供了VLA-4粘着途径在过敏原刺激之后从过敏绵羊的呼吸道开始的长时间炎症事件的病理生理指示剂(LAR和AHR)中起关键作用的有力证据。
表3
| 处理 | 剂量(mg) | 载体 | n | EAR(ΔSLR x h) | LAR(ΔSLR x h) | PC400(后/前) |
| 一天一次给药4天,在最后剂量之后24小时进行攻击 | ||||||
| PBSoMePUPA-V | 0.030.03 | EtOH:NSTris:NS | 844 | 4.33±0.811.53±0.34*1.40±0.35* | 4.96±0.400.59±0.16*0.02±0.06* | 0.38±0.031.06±0.04*1.04±0.04* |
绵羊,天性对猪蛔虫过敏,在重复每天给药阈下剂量oMePUPA-V或等量BPS 4天后24小时用猪蛔虫过敏原气溶胶攻击。肺力学,基于研究前基线值的特异性呼吸道阻力的变化报道,在过敏原攻击后测定了8个小时。早期呼吸道反应(0-4小时,EAR)和后期呼吸道反应(4-8小时,LAR)以特异性肺阻力曲线x时间的平均面积±标准误差表示。在研究开始之前和过敏原攻击后24小时测定对吸入的卡巴胆碱的呼吸道阻力。呼吸道反应性以攻击前和攻击后的PC400值(阻力增加到400%所需的卡巴胆碱的量)之比报道。
根据与对照组的多重比较的Dunnett试验,与PBS对照相比,单向方差分析*=p<0.05。这显示经统计EAR或LAR大大降低,或者与PBS对照组相比PC400比大大增加。
实施例3:
在延迟型高过敏性模型中的活性
绵羊红细胞研究
将来自Jackson实验室的8-19周龄的特定无病原体的雌性Balb/c小鼠用于所有试验。随意给这些动物喂食和水。每周从Charles River Pharm.Services(Southbridge,MA)获得来自相同绵羊的在Alsever溶液中的绵羊红细胞(sRBC)。在4℃下将该sRBC在1000g下离心造粒,除去任意可见血沉棕黄层。然后将这些细胞在生理盐水中冲洗。将这些细胞粒再悬浮于生理盐水中并用血细胞计数器计数。将这些细胞稀释于磷酸盐缓冲生理盐水(PBS)至2×108sRBC/mL。在第0天,通过皮下注射在100μLPBS中的2×107sRBC使小鼠致敏。在第5天,如上制备sRBC,但稀释在PBS中至最终浓度4×109sRBC/mL。在该制备中,将25μL皮下注射到右背足板中。
为了肠内给药化合物,将oMePUPA-V(Lot#2770-029)配制到在0.02MTRIS中的60%PEG 400的载体中至原料浓度为5mg/mL。在PEG/TRIS载体中制备适宜稀释液并通过肠道给药100μL。将抗-VLA-4抗体(PS/2)以浓度4.3mg/kg稀释到生理盐水中并通过腹膜内给药100μL。在用sRBC攻击之后立即给予所有处理。
在足背攻击20小时后使用来自Mitutoyo(Model#304-196,Dyer,Lancaster,PA)的张力测径规测定未被攻击的对照(左)和经过攻击的(右)背足板的膨胀。数据以足背厚度的变化表示,它是通过左后爪厚度减去右后爪厚度得到的。使用双尾Student’st-实验比较足背厚度的变化。
抗-VLA-4抗体PS/2以4.3mg/kg剂量腹膜内抑制膨胀约30%,而以20mg/kg剂量的肠内给药的oMePUPA-V在该模型中没有影响(未显示数据)。通过肠内途径以20mg/kg剂量给药oMePUPA-V到小鼠中sRBC诱导的DTH模型中的功效经研究,没有观察到功效。
实施例4.
延迟型过敏性模型中的活性
接触过敏性模型
将四个一笼放入Biogen无病毒动物家族中的微隔离器笼中并随意收到鼠食和自来水的20g雌性无病毒Balb/c小鼠(Jackson Laboratories,Bar Harbor,ME)用于所有研究中。将这些小鼠用氯胺酮∶赛拉嗪(90∶10mg/kg,腹膜内)麻醉。通过紧紧地刮屑皮毛暴露出一块3cm2的腹部皮肤、剑状耻骨,将该皮肤用70%乙醇冲洗干净。将体积为25μL在4∶1v/v丙酮∶橄榄油载体中的0.5%DNFB均匀地涂覆到该裸露的腹部皮肤上。用涂敷移液管尖轻轻抓破该皮肤以使其轻微发炎。将小鼠仰卧躺在其笼中,让其从麻醉中苏醒。开始致敏后24小时,再用25μL在载体中的0.5%DNFB在相同腹部皮肤位置致敏,然后再用移液管尖轻轻抓破。在束缚未被麻醉的小鼠的同时进行第二次致敏。在第5天(开始致敏后约120小时),使用低于刺激剂量的致敏物(在4∶1v/v丙酮∶橄榄油载体中的0.2%DNFB)攻击该免疫反应。用90∶10mg/kg氯胺酮∶赛拉嗪腹膜内注射将小鼠麻醉,将10μL 0.2%DNFB涂覆到左耳背面。右耳接受4∶1v/v丙酮∶橄榄油载体的相似涂覆。在接下来的24小时内,进行二相性耳膨胀反应,如图4所示。攻击后24小时,再用氯胺酮∶赛拉嗪将小鼠麻醉,用工程测微计测定两耳的厚度并精确到10-4英寸。
在第5天攻击该免疫反应之后4小时通过管饲法经口服给予化合物(100μL)或适宜载体(在等渗磷酸盐缓冲盐水[PBS]中的二甲亚砜[DMSO],100μL)。将每组8只小鼠的组用于每种试验处理。通过添加pH为8.8的0.5%磷酸钠缓冲液和3%DMSO将oMePUPA-V(Batch Number 2044-076)溶于蒸馏水中。以攻击后24小时其载体攻击的耳厚度和DNFB-攻击的耳厚度之差计算每只小鼠的耳膨胀反应。典型地DNFB诱导的耳膨胀为65-75×10-4英寸。通过将处理组与其载体对照组对比测定耳朵膨胀反应的抑制。使用遵循用于与对照组(Systat,SPSS Inc.)的多次对比的Dunnett试验的单向方差分析使用p<0.05评价处理组之间差异的统计显著性。值以平均值±平均值的标准误差(SEM)表示。
图4比较了在接受载体(DMSO,PBS)、正对照化合物(给以0.03μg/kg)或0.03或0.3mg/kg oMePUPA-V(DNFB攻击后4小时肠内给药(上方格))的小鼠中DNFB攻击后24小时测定的耳朵膨胀反应。在下方格中显示了处理诱导的抑制百分比。两种剂量的oMePUPA-V都显著地将耳朵膨胀反应抑制到通过正对照化合物显示的相似程度。
在DNFB攻击后4小时给的肠内0.03或0.3mg/kg单剂量的oMePUPA-V显著地抑制了小鼠接触过敏性模型中的耳朵膨胀反应。
实施例5:生物化学
5.1 在VCAM-Ig直接结合测定(DBA)中使用VCAM-Ig碱性磷酸酶共轭物测定oMePUPA-V的受体亲和性。
如所公开的构建并提纯VCAM-Ig(Jakubowski,A.等人,《细胞粘着和传染》3:131-142,1995)。为了裂解产色底物,如所公开的共轭到小牛肠内碱性磷酸酶上(Lobb,R.R.等人,《细胞粘着和传染》3:385-397,1995)。在人T细胞系Jurkat(α4β1)上评价VLA-4的结合。在有1mM Mn+2的情况下在这些细胞的表面上VCAM-Ig-AP和oMePUPA-V竞争结合到α4β1上。
在VCAM-Ig直接结合测定中,在有1mM MnCl2的情况下oMePUPA-V与VCAM-Ig-AP浓度依赖性地以8±1nM(n=9)的IC50竞争结合到Jurkat细胞上。
5.2 在纯化VLA-4蛋白质/蛋白质测定中使用VCAM-Ig碱性磷酸酶共轭物测定oMePUPA-V的受体亲和性。
从α4-转染的K562细胞的高表达亚克隆的洗涤剂提取物中通过抗体亲和性色谱法提纯VLA-4并将其固定在微量滴定孔上建立蛋白质/蛋白质竞争性结合测定。在没有或有oMePUPA-V(Lot#2)和1mM MnCl2的情况下将VCAM-Ig-AP结合到提纯的VLA-4-涂布板上。在405nm下读板并使用SoftMax v.2.32软件分析该数据。
VCAM-Ig共轭物与提纯VLA-4的结合完全被特异性中和抗-α4单克隆抗体(HP1/2)阻断。在VLA-4蛋白质/蛋白质测定中由oMePUPA-V获得的两个IC50值列于表4中,它是由VCAM-Ig-AP竞争性结合测定和CS1细胞粘着测定在Jurkat细胞上获得的IC50′s。
5.3 在CS1细胞粘着测定中评价oMePUPA-V的受体亲和性
a.Jurkat细胞粘着在CS1/BSA共轭物上
合成肽NH2-半胱氨酸-酪氨酸-CS-1并以CS1/BSA比为10∶1将其偶合到BSA-SMCC(SMCC是与BSA和合成肽的单独半胱氨酸上的游离氨基反应的异型双功能交联剂)上。用稀释至最终浓度为1μg/ml的100μL共轭物将孔涂布一夜。第二天用PBS中的BSA将这些孔阻塞1小时,然后将其冲洗3次。
将人T细胞系Jurkat用2μM BCECF-AM标记,该BCECF-AM为一种荧光染料(2′,7′,二-(2-羧乙基)-5和-6)羧基荧光黄乙酰氧基甲酯(Molecular Probes Inc.,Eugene,Oregon;catalog #B-1150),其经内在化和去酯化将该染料捕获在肝细胞中。将含1mM Mn+2的缓冲剂中的Jurkat细胞(1×105个细胞/孔)加入含有三倍系列抑制剂稀释液的涂布板中。一式两份测定每一浓度。室温下30分钟后,将这些板颠倒并冲洗3次或者直到没有细胞粘着在仅用BSA涂布的对照孔中。在Cytofluor荧光板读数仪中使用485nm的兴奋波长和530nm的发射波长将CS-1粘着细胞定量。
在没有化合物的情况下粘着在CS1/BSA的细胞用作0%抑制对照,同时将仅粘着在BSA上的细胞用作100%抑制对照。使用Deltagraph软件第5版计算IC50′s。
在有Mn+2的情况下标记Jurkat细胞的粘着被EDTA和中和抗-α4β1mAb,HP1/2,完全阻断,这说明结合是特异性的。表4给出了oMePUPA-V在CS1/BSA粘着测定中的活性以及结合测定结果。
oMePUPA-V是含Mn+2的缓冲剂中VLA-4的有效拮抗物。当在有Mn+2的情况下将其在分离VLA-4上测定时比在结合测定中在Jurkat细胞上测定的有效性高出80倍。通过其剂量依赖性地并完全阻断Jurkat粘着在CS1上的能力证实,oMePUPA-V为功能性拮抗物。在粘着测定中的绝对值大于在结合测定中观察到的。这可能是由于粘着的多价性能。在所有测定形式中,EDTA和HP1/2的结合抑制证明特异性地结合到VLA-4上。
表4:在有1mM MnCl2的情况下在VCAM-Ig竞争性结合测定、CS1细胞粘着测定和提纯VLA-4蛋白质/蛋白质测定中测定的oMePUPA-V的受体亲和性
| IC50±SD[nM] | |
| 测定 | oMePUPA-V |
| Jurkat细胞VCAM-Ig结合 | 8±1(n=9) |
| Jurkat细胞CS1粘着 | 22±2(n=4) |
| 提纯的VLA-4VCAM-Ig结合 | 0.1(n=9)(0.1,0.1) |
6.4 oMePUPA-V抑制的特异性
a.使用JY细胞在VCAM-Ig直接结合和CS1粘着测定中评价oMePUPA-V的特异性
在有Mn+2的情况下在JY细胞上测定与α4β1的结合。在结合测定中,在JY细胞上VCAM-Ig和oMePUPA-V竞争结合到α4β1上(参见测定方案的段4.1.1)。在该细胞粘着测定中,试验0MePUPA-V阻断JY(α4β1)细胞结合到CS1/BSA共轭物上的能力。
oMePUPA-V不阻断α4β1结合到VCAM-Ig或CS1/BSA上。抗-β7Mab、Fib27(Pharmingen)完全抑制这些相互作用,这说明结合上α4β1特异性的。因此oMePUPA-V为VLA-4特异性抑制剂。结果列于表5中。
b.使用K562细胞粘着到涂布有Fn-120的孔上评价oMePUPA-V的特异性
将未处理的96孔聚苯乙烯平底板用5μg/ml Fn-120在4℃下涂布一夜。将这些板用磷酸盐缓冲盐水(PBS)冲洗2次,并在室温下用1%牛血清白蛋白(BSA)堵塞1小时。将这些板用含1mM MnCl2的TBS缓冲液(测定缓冲液)冲洗2次。K562细胞用2μM荧光染料BCECF-AM标记(参见段4.1.3),并将其在室温下经过30分钟结合到板上。将这些板颠倒并冲洗3次,在Cytofluor荧光板读数仪中使用485nm的兴奋波长和530nm的发射波长将粘着细胞定量。
K562与Fn-120的粘着完全被中和抗-α5抗体IIA1(Pheamingen)阻断,这说明通过VLA-5的特异性结合。oMePUPA-V的剂量高至100μM也没有抑制K562细胞结合到Fn120K上。参见下表5。
c.进行聚集测定评价oMePUPA-A的特异性
方法
使用富含血小板的血浆通过标准血小板聚集评价抗gpIIbIIIa的活性。使用ADP在血浆中开始聚集,其中Ca+2和Mg+2为主要二价阳离子。将GRGDSP@100μg/mL用作正对照。
结果
以三个剂量1、10和100μM测定oMePUPA-A。在选择剂量下通过ADP诱导没有抑制血小板聚集。结果列于表5中。oMePUPA-A对VLA-4高度特异性(>10000倍)。它没有抗相关整联蛋白α4β7和VLA-5或抗β3整联蛋白gpIIbIIIa的可测量活性(>100μM)。
表5:在α4β7 VCAM-Ig竞争性结合测定、α4β7和VLA-5粘着测定、以及血小板聚集研究中测定的oMePUPA-V的抑制活性
| 细胞系 | 配体 | 二价阳离子 | oMePUPA-VIC50±SD[nM] |
| JY | VCAM-Ig | Mn+2 | 3%抑制 |
| (α4β7) | DBA | @100μM(n=3) | |
| JY(α4β7) | CS1/BSA粘着 | Mn+2 | 没有抑制@100μM(n=4) |
| K562(VLA-5) | Fn-120粘着 | Mn+2 | 没有抑制@100μM(n=3) |
| 血小板(IIbIIIa) | 纤维蛋白原聚集 | Ca+2/Mn+2 | 没有抑制@100μM(n=1) |
实施例6:LIBS诱导的oMePUPA-V测定
6.1使用LIBS抗体9EG7在Jurkat上测定
a.在体外通过FACS分析测定α4β1拮抗物的LIBS诱导。在37℃下用仅含2mM MgCl2(Mg+2-TBS)的TRIS缓冲盐水或试验化合物的系列稀释液将Jurkat细胞(2×105/孔)预培养20分钟。将这些样品转移到冰浴中并以10μg/ml的最终浓度补充LIBS抗体9EG7。将这些细胞用Mg+2-TBS冲洗2次并将其再悬浮于在Mg+2-TBS中的1∶200稀释的FITC共轭羊抗大鼠IgG中并在4℃下培养30分钟。将这些细胞冲洗2次并再悬浮于Mg+2-TBS中。通过FACS分析(Becton Dickinson FACScan)测定平均荧光强度(MFI)。结果以MFI表达。通过Microsoft Excel 5.0版和Deltagraph 4.0版软件分析数据。
图5显示了与2mM Mg+2缓冲液(方格B)相比的oMePUPA-V诱导的LIBS表位的暴露。该诱导为浓度依赖型并与用1mM Mg+2(方格A)观察到的诱导非常相似。省略LIBS抗体和检测抗体,或者仅省略抗体消除了贴标签(方格B)。该反应的ED50为-20nM。
结论
这些数据说明,oMePUPA-A诱导VLA-4中与用天然配体观察的相同构象改变。LIBS值一般落入oMePUPA-V结合和粘着测定所定义的范围(分别为8nM和22nM)内。
6.2 多种类受体筛选
a.在VCAM-Ig直接结合测定中使用VCAM-Ig碱性磷酸酶共轭物和来自不同种的周围血液淋巴细胞或脾细胞测定oMePUPA-V的受体亲和性。
PBL,使用绵羊PBL(Abraham,W.M.等人J.Clin.Invest.93:776-787,1994)中所述的方法从人、绵羊和狗的外周血液中分离出来。使用VCAM-Ig-AP竞争性结合测定比较oMePUPA-V在这些不同细胞类型上的结合。
由oMePUPA-V在有Mn+2的情况下在来自不同种的外周血液淋巴细胞或脾细胞上获得的IC50′s示于表6中。在有Mn+2的情况下,具有相似IC50的oMePUPA-V抑制VCAM-Ig结合到从人、大鼠、狗、绵羊和小鼠中获得的淋巴细胞上。没有证据表明种特异性。这与在种中观察到的VLA-4和其天然配体、CS-1和VCAM的序列保守高度一致。
表6:在使用VCAM-Ig碱性磷酸酶共轭物和来自不同种的处周血液淋巴细胞或脾细胞在VCAM-Ig竞争性结合测定中测定的oMePUPA-V的受体亲和性
| 种 | 源 | 二价阳离子 | IC50[nM] |
| 人 | PBL | Mn+2 | 6±1(n=3) |
| 绵羊 | PBL | Mn+2 | 3±1(n=3) |
| 狗 | PBL | Mn+2 | 13±2(n=3) |
| 小鼠 | 脾细胞 | Mn+2 | 4±2(n=4) |
| 大鼠 | 脾细胞 | Mn+2 | 5±1(n=3) |
实施例7:oMePUPA-V的受体动力学
7.1 使用3H-已知的抑制剂作探针的竞争性测定
在组织培养保温箱中在37℃下将Jurkat保持在PRMI-1640培养基+10%胎牛血清中。为了结合研究,通过离心将这些细胞造粒,用TBS(50mMTris HCl,150mM NaCl,0.1%牛血清白蛋白,2mM葡萄糖,10mM HEPESpH7.4)冲洗2次,以约2×106个细胞/ml悬浮于TBS中,并使用Neubauer血细胞计数器计数。在指定缓冲液中将这些细胞进一步稀释至1.5×106/ml,并经受每个试验所定义的特定处理。然后通过离心将这些细胞造粒,将其再悬浮于100μl试验缓冲液中,并转移到含2.9mlScintiVerse II(Fisher Scientific)的闪烁小瓶中。通过闪烁计数计量细胞相关的放射性。在这些条件下结合的计数测定未被试验化合物占领并因此没有结合到该3H-已知的抑制剂的整联蛋白。在硅化处理的1.5ml微量离心管中用标准1ml样品进行所有研究。3H-已知的抑制剂在细胞(本底物)上的非特异性结合通过测定在没有金属离子的情况下结合的抑制剂来定义。通过结合总计数减去非特异性计数计算结合的特异性计数。
进行一系列竞争性研究以验证oMePUPA-V和已知抑制剂对VLA-4上的相同位置的竞争。首先,将3H-已知的抑制剂与等摩尔量的oMePUPA-V、10倍量和100倍量混合,用Jurkat细胞培养并评价冷抑制剂竞争结合已知抑制剂的能力。oMePUPA-V处理产生3H-已知的抑制剂结合的剂量依赖性抑制。竞争3H-已知的抑制剂结合所需的oMePUPA-V的浓度比将冷却用作竞争剂时的大10倍,与Mn+2-激活的VLA-4的较低亲和性一致。其次,Mn+2-激活的Jurkat细胞用3H-已知的抑制剂处理,以便首先占领带有放射性探针的VLA-4,然后加入过量冷oMePUPA-V。接下来用过量冷oMePUPA-V或已知抑制剂的处理不能辨别出其替换放射性探针的能力。第三,Mn+2-激活的Jurkat细胞用饱和量的oMePUPA-V处理,并且测定该oMePUPA-V分离的速度,与用于Mn+2-激活的VLA-4的已知抑制剂的延长半衰期不同,oMePUPA-V以不到10分钟的t1/2很快从oMePUPA-V-VLA-4释放。oMePUPA-V和已知抑制剂的t1/2的很大差异暗示,oMePUPA-V对VLA-4的较低亲和性结果导致其更快的分离速度。
分离数据证实,oMePUPA-V与VLA-4的结合特别依赖于VLA-4的活化状态,并且它呈现用已知抑制剂看到的相同的活化选择性。至于Mn+2-激活的VLA-4,oMePUPA-V从Mn+2-激活的VLA-4分离的t1/2比在竞争形式中能够测定的最短时间点少10分钟。另一方面,在有Mn+2和活化抗体TS2/16的情况下,t1/2延长(20分钟)。还没有详细评价所有可能的活化状态,然而可以设计快速高亮度差别的简单筛选。在该试验中,将固定浓度的oMePUPA-V(10nM)与5nM3H-已知的抑制剂混合,并在这些条件下以不同活化状态进行结合。如果oMePUPA-V对VLA-4具有异常高或低的亲和力,那么人们将通过3H-已知的抑制剂的量的区别检测它。在不同活化条件下结合的3H-已知的抑制剂的百分比的差异近似地可以该抑制剂的已知性能为基础预测。
结合研究证实oMePUPA-V以与其亲和性一致的浓度与已知抑制剂竞争结合到VLA-4上,并证实这两种化合物竞争整联蛋白的相同位置。在不同VLA-4活化状态下oMePUPA-V和已知抑制剂结合的相似性暗示结合机理相似。
7.2 在Panlabs和Cerep筛选中测定oMePUPA-V
在Panlabs轮廓筛、发现筛和放射性配体、酶和功能性测定的免疫筛板中以及Cerep膜受体板中试验oMePUPA-V。在包括NK1受体测定的所有测定中10μM的oMePUPA-V观察不到显著活性,相反已知抑制剂显示一些活性。Cerep还报道oMePUPA-V没有显示出抑制人ACE蛋白酶活性。ACE蛋白酶源为人内皮细胞(HUVEC)。3H-HGG,将其添加到HUVEC中,被ACE转变成3H-马尿酸和双甘氨肽。卡托普利,一种有效的ACE抑制剂,以990pM的IC50阻断该转化,然而10μM的oMePUPA-V不能。
药物性质:
oMePUPA-V为白色至黄白色结晶粉末。溶于DMSO并具有0.120mg/mL的水溶性。通过DSC、TGA和热阶段显微镜检查研究的oMePUPA-V热行为显示,该物质在约160℃下熔化。在约136℃,DSC和TGA分析暗示,oMePUPA-V失去可能与水合物脱水一致的挥发性杂质。
制剂
雾化制剂
100mL 5mg/mL的oMePUPA-V雾化制剂的生产说明如下。
如下制备200mL缓冲原液:
1、称重0.286g USP级氨丁三醇,加入适宜容器中。
2、称重1.676g USP级氯化钠,加入相同容器中。
3、加入200mL USP级注射用水。
混合直到均匀。
1、称重0.500g oMePUPA-V并加入适宜容器。
2、加入步骤1中制备的100mL缓冲液。
3、混合直到均匀。
4、无菌过滤到适宜容器中。
5、用适宜封口措施密封。
典型制剂性质:
pH:7.4,渗重量摩尔浓度:290mOsm
实施例9:
稳定性指示HPLC步骤
柱:ZorbaxSB-C18,3μm颗粒,4.6×150mm
保护柱:ZorbaxSB-C18,5μm颗粒,4.6×12.5mm
流速:1mL/分钟
柱温:40℃
流动相A:0.1%(w/v)水中的三氟乙酸(TFA)
B:0.1%(w/v)在90%(v/v)乙腈、10%(v/v)水中的TFA组分:
时间(分钟)
%B
0-3 15
3-18 15-100
18-21 100
21-28 15
注射:10μL在Tris/NaCl/水(散装中间体)中或在0.1%TFA/45%乙腈(最终产物)中的0.2mg/mL溶液。
检测:UV 254nm(开始)和215nm
对照:oMePUPA-V,在沸水中加热20分钟。
完成开始方法的定量。
药物稳定性
在以下贮藏条件下贮藏2周后在散装中间体中没有观察到降解:在密封小瓶中40℃;在密封小瓶中50℃;在25℃、RH60%下;和在40℃、RH75%下。在4周后,在40℃或50℃下可以检测出一个或者两个降解峰,但是每个杂质峰的水平仍然低于0.02%。
水溶性
a)雾化制剂,在Tris/NaCl中5mg/mL,在室温下贮藏2个月,早期显示出总水平1%(254nm)和2-3%(215nm)的洗脱降解峰。
b)在沸水中将雾化制剂加热20分钟,在254nm纯度由99.9%降到98.7%,在215nm纯度由100%降到93.6%。
c)在Tris/NaCl/水中的0.2mg/mL溶液在中性pH下在2-8℃下至少稳定1周。
显而易见,本领域技术人员在不背离本发明的宗旨或范围的情况下可以对本发明进行各种改进和变化。因此,本发明覆盖了附加权利要求书及其等价范围内的本发明提供的这些改进和变化。
Claims (12)
1.一种细胞粘着抑制化合物
oMePUPA-V
及其药物上可接受的酯、药物上可接受的盐或其异构体。
2.药物组合物,其含有权利要求1的化合物和药物上可接受的载体。
3.权利要求2的药物组合物,还含有选自皮质类固醇、支气管扩张药、平喘药、消炎药、抗风湿剂、免疫抑制剂、抗代谢物、免疫调制剂、抗牛皮癣药和治疗糖尿病药的第二种试剂。
4.药物组合物,其含有权利要求1的化合物和一种或多种VLA-4介导的细胞粘着抑制剂化合物。
5.权利要求1的化合物用于制备预防、抑制或减少VLA-4介导的细胞粘着的药物的用途。
6.权利要求1中的化合物用于制备预防、抑制或减少炎症药物的用途。
7.权利要求1的化合物用于制备治疗哺乳动物中哮喘、过敏性鼻炎、多发性硬化、动脉粥样硬化、炎性肠病或多发性骨髓瘤的药物的用途。
8.权利要求1的化合物用于制备治疗多发性硬化的药物的用途。
9.权利要求1的化合物用于制备治疗炎性肠病的药物的用途。
10.含有权利要求1的化合物的酯的药物组合物。
11.权利要求10的组合物,其中所述酯是由权利要求1中的化合物与选自甲醇、乙醇、丙醇、丁醇和直链或支链烷基C1-C10的醇反应制得的。
12.权利要求1的化合物用于制备治疗、预防或改善哮喘症状的药物的用途。
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| US7618630B2 (en) | 1998-09-14 | 2009-11-17 | Board Of Regents, The University Of Texas System | Methods of treating multiple myeloma and myeloma-induced bone resorption using integrin antagonists |
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