Underwood D J, Green B G, Chabin R, Mills S, Doherty J B, Finke P E, MacCoss M, Shah S K, Burgey C S, Dickinson T A
Department of Enzymology, Merck Research Laboratories, Rahway, New Jersey 07065, USA.
Biochemistry. 1995 Nov 7;34(44):14344-55. doi: 10.1021/bi00044a011.
A combination of NMR spectroscopy and electrospray ionization mass spectrometry (ESI-MS) was used to probe the identity of beta-lactam-derived complexes with serine proteases. The carbon and proton NMR chemical shifts of the human leucocyte elastase (HLE)-inhibitor complex derived from [4-13C]-L-680,833, [S-(R*,S*)]-4-[(1-(((1-(4- methylphenyl)butyl)amino)carbonyl)-3,3-diethyl-2-oxo-4- azetidinyl)oxy]benzeneacetic acid, were consistent with an sp3 hybridized carbon. The ESI-MS spectrum of the L-680,833-derived HLE-I complex indicated an increase of 333 Da over the mass of the free enzyme. The data are consistent with acylation of the active site serine, loss of p-hydroxybenzeneacetic acid, and formation of a carbinolamine at the carbon deriving from C-4 of the lactam ring. The complexes produced from HLE and the diastereomers of L-680,833 display identical masses. Since the 4R-isomers produce more stable complexes [Green et al. (1995) Biochemistry 34, 14331-14343], these data suggest that these complexes differ in their stereochemistry or conformation. The structural model of the HLE-I complexes derived from the diastereomers predicts that the hydroxyl of the carbinolamine derives from a structurally observed water molecule yielding S-stereochemistry in all cases. In this model, the 4S- and 4R-diastereomers produce complexes that differ by the location of the side chain of a phenylalanine residue. The mass of HLE was increased by that of L-684,481, (R)-1-(((1-(4-methylphenyl)butyl)amino)carbonyl)-3,3-diethyl-2-azetidino ne, which lacks a leaving group at C-4 in the complex derived from this compound. L-691,886, [S-(R*,S*)]-4-[(1-(((1-(4-ethoxyphenyl)butyl)amino)carbonyl)- 3,3-diethyl-4-oxo-2-azetidinyl)-oxy]benzeneacetic acid, produces two complexes of different mass that reactivate with different rates. The mass of the less stable complex is consistent with the acyl-enzyme of 2,2-ethyl-3-oxopropanoic acid while the mass of the more stable complex is analogous to the carbinolamine observed during L-680,833 inactivation. Porcine pancreatic elastase (PPE) produces a complex with a mass consistent with replacement of the C-4 leaving group by water to produce a carbinolamine from L-684,248, [S-(R*,S*)]-4-[(1-(((1-(4-methylphenyl)butyl)amino)carbonyl)-3,3-dimethy l - 2-oxo-4-azetidinyl)oxy]benzoic acid. The C-4 diastereomer, L-684,249, produces two PPE-I complexes with different masses. One of these complexes has a mass identical to the mass of the complex derived from L-684,248 while the mass of the other complex indicates the presence of the entire inhibitor molecule.(ABSTRACT TRUNCATED AT 400 WORDS)
采用核磁共振光谱法和电喷雾电离质谱法(ESI-MS)相结合的方法,探究β-内酰胺衍生的与丝氨酸蛋白酶形成的复合物的特性。源自[4-¹³C]-L-680,833,即[S-(R*,S*)]-4-[(1-(((1-(4-甲基苯基)丁基)氨基)羰基)-3,3-二乙基-2-氧代-4-氮杂环丁烷基)氧基]苯乙酸的人白细胞弹性蛋白酶(HLE)-抑制剂复合物的碳和质子核磁共振化学位移,与sp³杂化碳一致。源自L-680,833的HLE-I复合物的ESI-MS谱表明,其质量比游离酶的质量增加了333 Da。这些数据与活性位点丝氨酸的酰化、对羟基苯乙酸的损失以及在内酰胺环C-4衍生的碳上形成氨基醇一致。由HLE和L-680,833的非对映异构体产生的复合物显示出相同的质量。由于4R-异构体产生更稳定的复合物[格林等人(1995年),《生物化学》34卷,14331 - 14343页],这些数据表明这些复合物在立体化学或构象上存在差异。源自非对映异构体的HLE-I复合物的结构模型预测,氨基醇的羟基源自结构上观察到的水分子,在所有情况下都产生S-立体化学。在该模型中,4S-和4R-非对映异构体产生的复合物因苯丙氨酸残基侧链位置的不同而有所差异。L-684,481,即(R)-1-(((1-(4-甲基苯基)丁基)氨基)羰基)-3,3-二乙基-2-氮杂环丁烷,在由此化合物衍生的复合物中C-4处缺乏离去基团,它使HLE的质量增加。L-691,886,即[S-(R*,S*)]-4-[(1-(((1-(4-乙氧基苯基)丁基)氨基)羰基)-3,3-二乙基-4-氧代-2-氮杂环丁烷基)-氧基]苯乙酸,产生两种质量不同且以不同速率重新活化的复合物。较不稳定复合物的质量与2,2-乙基-3-氧代丙酸的酰基酶一致,而较稳定复合物的质量类似于在L-680,833失活过程中观察到的氨基醇。猪胰弹性蛋白酶(PPE)与一种质量一致的复合物,该复合物是由L-684,2,48,即[S-(R*,S*)]-4-[(1-(((1-(4-甲基苯基)丁基)氨基)羰基)-3,3-二甲基-2-氧代-4-氮杂环丁烷基)氧基]苯甲酸中的C-4离去基团被水取代而产生氨基醇形成的。C-4非对映异构体L-684,249产生两种质量不同的PPE-I复合物。其中一种复合物的质量与源自L-684,248的复合物质量相同,而另一种复合物的质量表明存在整个抑制剂分子。(摘要截选至400字)
