Lindigkeit R, Biller A, Buch M, Schiebel H M, Boppré M, Hartmann T
Institut für Pharmazeutische Biologie, Technische Universität Braunschweig, Germany.
Eur J Biochem. 1997 May 1;245(3):626-36. doi: 10.1111/j.1432-1033.1997.00626.x.
Larvae of Creatonotos transiens (Lepidoptera, Arctiidae) and Zonocerus variegatus (Orthoptera, Pyrgomorphidae) ingest 14C-labeled senecionine and its N-oxide with the same efficiency but sequester the two tracers exclusively as N-oxide. Larvae of the non-sequestering Spodoptera littoralis eliminate efficiently the ingested alkaloids. During feeding on the two alkaloidal forms transient levels of senecionine (but not of the N-oxide) are built up in the haemolymph of S. littoralis larvae. Based on these results, senecionine [18O]N-oxide was fed to C. transiens larvae and Z. variegatus adults. The senecionine N-oxide recovered from the haemolymph of the two insects shows an almost complete loss of 18O label, indicating reduction of the orally fed N-oxide in the guts, uptake of the tertiary alkaloid and its re-N-oxidation in the haemolymph. The enzyme responsible for N-oxidation is a soluble mixed function monooxygenase. It was isolated from the haemolymph of the sequestering arctiid Tyria jacobaeae and purified to electrophoretic homogeneity. The enzyme is a flavoprotein with a native Mr of 200000 and a subunit Mr of 51000. It shows a pH optimum at 7.0, has its maximal activity at a temperature of 40-45 degrees C and an isoelectric point at pH 4.9. The reaction is strictly NADPH-dependent (Km 1.3 microM). From 20 pyrrolizidine alkaloids so far tested as substrates, the enyzme N-oxidizes only alkaloids with structural elements which are essential for hepatotoxic and genotoxic pyrrolizidine alkaloids (i.e. 1,2-double bond, esterification of the allylic hydroxyl group, presence of a second free or esterified hydroxyl group at carbon 7). A great variety of related alkaloids and xenobiotics were tested as substrate, none was accepted. The Km values of senecionine, monocrotaline and heliotrine, representing the three main types of pyrrolizidine alkaloids, are 1.3 microM, 12.5 microM and 290 microM, respectively. The novel enzyme was named senecionine N-oxygenase (SNO). The enzyme was partially purified from two other arctiids. The three SNOs show the same general substrate specificity but differ in their affinities towards the main structural types of pyrrolizidine alkaloids. The enzymes from the two generalists (Creatonotos transiens and Arctia caja) display a broader substrate affinity than the enzyme from the specialist (Tyria jacobaeae). The two molecular forms of pyrrolizidine alkaloids, the lipophilic protoxic tertiary amine and its hydrophilic nontoxic N-oxide are discussed in respect to their bioactivation and detoxification in mammals and their role as defensive chemicals in specialized insects. Pyrrolizidine-alkaloid-sequestering insects store the alkaloids as nontoxic N-oxides which are reduced in the guts of any potential insectivore. The lipophilic tertiary alkaloid is absorbed passively and then bioactivated by cytochrome P-450 oxidase.
瞬态客夜蛾(鳞翅目,灯蛾科)和杂色稻蝗(直翅目,锥头蝗科)的幼虫以相同效率摄取14C标记的千里光碱及其N-氧化物,但仅将这两种示踪剂隔离为N-氧化物。非隔离性的斜纹夜蛾幼虫能有效消除摄入的生物碱。在取食这两种生物碱形式时,斜纹夜蛾幼虫的血淋巴中会短暂积累千里光碱(而非N-氧化物)。基于这些结果,将千里光碱[18O]N-氧化物投喂给瞬态客夜蛾幼虫和杂色稻蝗成虫。从这两种昆虫的血淋巴中回收的千里光碱N-氧化物显示18O标记几乎完全丢失,这表明口服的N-氧化物在肠道中被还原,叔胺生物碱被吸收并在血淋巴中再次N-氧化。负责N-氧化的酶是一种可溶性混合功能单加氧酶。它是从隔离性灯蛾科昆虫欧洲粉斑螟的血淋巴中分离出来的,并纯化至电泳纯。该酶是一种黄素蛋白,天然分子量为200000,亚基分子量为51000。其最适pH为7.0,在40 - 45摄氏度温度下具有最大活性,等电点为pH 4.9。该反应严格依赖NADPH(Km为1.3微摩尔)。在迄今为止测试的20种吡咯里西啶生物碱底物中,该酶仅对具有对肝毒性和基因毒性吡咯里西啶生物碱至关重要的结构元件的生物碱进行N-氧化(即1,2-双键、烯丙基羟基的酯化、碳7位存在第二个游离或酯化羟基)。测试了多种相关生物碱和异生物质作为底物,均未被接受。代表三种主要吡咯里西啶生物碱类型的千里光碱、农吉利碱和天芥菜碱的Km值分别为1.3微摩尔、12.5微摩尔和290微摩尔。这种新酶被命名为千里光碱N-加氧酶(SNO)。该酶从另外两种灯蛾科昆虫中部分纯化得到。这三种SNO显示出相同的一般底物特异性,但对吡咯里西啶生物碱主要结构类型的亲和力不同。来自两种多食性昆虫(瞬态客夜蛾和榆绿天蛾)的酶比来自专食性昆虫(欧洲粉斑螟)的酶表现出更广泛的底物亲和力。讨论了吡咯里西啶生物碱的两种分子形式,即亲脂性的原生毒性叔胺及其亲水性的无毒N-氧化物在哺乳动物中的生物活化和解毒作用,以及它们作为特殊昆虫防御性化学物质的作用。吡咯里西啶生物碱隔离性昆虫将生物碱储存为无毒的N-氧化物,在任何潜在食虫动物的肠道中被还原。亲脂性叔胺生物碱被被动吸收,然后由细胞色素P-450氧化酶进行生物活化。
