Actions of two serine proteases from Trimeresurus jerdonii venom on chromogenic substrates and fibrinogen

Jerdonobin and jerdofibrase are two serine proteases purified from the venom of Trimeresurus jerdonii. The Michaelis constant K-m and the catalytic rate constant K-cat of jerdonobin or jerdofibrase on three chromogenic substrates, H-D-Pro-Phe-Arg-pNA (S2302), H-D-Phe-pipecolyl-Arg-pNA (S2238), and H-D-Val-Leu-Lys-pNA (S2251) were obtained from lineweaver-Burk plots. Jerdofibrase could hydrolyze all three substrates, but jerdonobin had no detectable activity on S2251, suggesting a relatively broader substrate specificity for jerdofibrase than jerdonobin. By SDS-PAGE, jerdofibrase preferentially degraded Bbeta-chain of fibrinogen. It also degraded Aalpha-chain of fibrinogen with relatively slow activity, but did not act on the gamma-chain. In contrast, jerdonobin did not degrade fibrinogen within 12 h. Fibrinopeptides liberation test, identified by HPLC, showed jerdonobin released fibrinopeptide A and a small amount of fibrinopeptide B. Unlike jerdonobin, jerdofibrase mainly released fibrinopeptide B. These results indicate that the two enzymes differ in their ability to hydrolyze chromogenic substrates and in their actions on fibrinogen. (C) 2002 Elsevier Science Inc. All rights reserved.

Biochemical and biological properties of Trimeresurus jerdonii venom and characterization of a platelet aggregation-inhibiting acidic phospholipase A(2)

Several biochemical and biological activities such as phospholipase A(2), arginine esterase, proteolytic, L-amino acid oxidase, 5'nucleotidase, acetylcholinesterase, thrombin-like, anticoagulant, and hemorrhagic activities were determined for whole desiccated venom of Trimeresurus jerdonii. An acidic phospholipase (named TJ-PLA(2)) was purified by anionic exchange chromatography, gel filtration, and reverse phase HPLC. TJ-PLA(2) had a molecular weight of 16,000 and a pI of 4.8. TJ-PLA(2) was non-lethal to mice up to an i.p. dose of 15 mg/kg body weight and lacked neurotoxicity and myotoxicity. It induced edema in the footpads of mice. The purified enzyme inhibited ADP- and collagen-induced human platelet aggregation in a manner which was both dose- and time-dependent.

N49 phospholipase A(2), a unique subgroup of snake venom group II phospholipase A(2)

A novel phospholipase A(2) (PLA(2)) with Asn at its site 49 was purified from the snake venom of Protobothrops mucrosquamatus by using SP-Sephadex C25, Superdex 75, Heparin-Sepharose (FF) and HPLC reverse-phage C-18 chromatography and designated as TM-N49

Jerdonase, a novel serine protease with kinin-releasing and fibrinogenolytic activity from Trimeresurus jerdonii venom

A novel kinin-releasing and fibrin (ogen)olytic enzyme termed jerdonase was purified to homogeneity from the venom of Trimeresurus jerdonii by DEAE Sephadex A-50 anion exchange, Sephadex G-100 (superfine) gel filtration and reverse-phase high performance liquid chromatography (RP-HPLC). Jerdonase migrated as a single band with an approximate molecular weight of 55 kD under the reduced conditions and 53 kD under the non-reduced conditions. The enzyme was a glycoprotein containing 35.8% neutral carbohydrate. The N-terminal amino acid sequence of jerdonase was determined to be IIGGDECNINEHPFLVALYDA, which showed high sequence identity to other snake venom serine proteases. Jerdonase catalyzed the hydrolysis of BAEE, S-2238 and S-2302, which was inhibited by phenymethylsulfonyl fluoride (PMSF), but not affected by ethylenediaminetetraacetic acid (EDTA). Jerdonase preferentially cleaved the Aalpha-chain of human fibrinogen with lower activity towards Bbeta-chain. Moreover, the enzyme hydrolyzed bovine low-molecular-mass kininogen and releasing bradykinin. In conclusion, all results indicated that jerdonase was a multifunctional venom serine protease.

A novel serine protease inhibitor from Bungarus fasciatus venom

By Sephadex G-50 gel filtration, cation-exchange CM-Sephadex C-25 chromatography and reversed phase high-performance liquid chromatography (HPLC), a novel serine protease inhibitor named bungaruskunin was purified and characterized from venom of Bungarus fasciatus. Its cDNA was also cloned from the cDNA library of B. fasciatus venomous glands. The predicted precursor is composed of 83 amino acid (aa) residues including a 24-aa signal peptide and a 59-aa mature bungaruskunin. Bungaruskunin showed maximal similarity (64%) with the predicted serine protease inhibitor blackelin deduced from the cDNA sequence of the red-bellied black snake Pseudechis porphyriacus. Bungaruskunin is a Kunitz protease inhibitor with a conserved Kunitz domain and could exert inhibitory activity against trypsin, chymotrypsin, and elastase. By screening the cDNA library, two new B chains of beta-bungarotoxin are also identified. The overall structures of bungaruskunin and beta -bungarotoxin B chains are similar; especially they have highly conserved signal peptide sequences. These findings strongly suggest that snake Kunitz/BPTI protease inhibitors and neurotoxic homologs may have originated from a common ancestor. (c) 2007 Elsevier Inc. All rights reserved.

异硫氰酸苯酯衍生化法测定微透析样品中氨基酸的方法

本发明涉及一种异硫氰酸苯酯衍生化法测定脑内透析样品中氨基酸的方法，属生物医学领域。该方法由样品的采集(即脑内微透析)、样品的衍生和干燥以及HPLC分离等组成。实验前一周，在动物特定部位埋植透析导管。待恢复后，安装透析探针，并以一定流速灌流人工脑脊液，间隔一定时间收集一次透析样品。然后，在样品中加入一定量的内标试剂，经冷冻干燥、异硫氰酸苯酯衍生、再干燥、稀释等步骤处理后，样品经反相HPLC洗脱，紫外检测。本发明具有简便快速、衍生产物稳定、分析时间短、化学选择性和分析灵敏度高(可达1pmol)、一、二级氨基酸均可检测的分析方法，由此可实现微透析与反相高压液色谱紫外检测技术结合对脑内痕量活性物质的动态监测。

中华眼镜蛇蛇毒神经生长因子生物活性和理化性质测定

目的：控制中华眼镜蛇蛇毒神经生长因子产品质量，研究其理化性质及生物学活性的定性和定量。方法：通过离子交换色谱、凝胶过滤及FPLC色谱分高纯化得到中华眼镜蛇蛇毒神经生长因子，按国家新药审批有关要求对其进行了SDS－PAGE电泳，N端蛋白质序列规定，HPLC色谱分析，UV光谱图谱扫描，并利用PC12细胞培养法和鸡胚背根神经节培养法检测其生物活性。结果：电泳为一条带，亚基分子量为13500，N端蛋白质序列测定后确证为神经生长因子（NGF），HPLC为单峰，相对百分含量为95％以上，279．6nm处呈现出蛋白质样特征吸收峰。生物活性测定为，PC12细胞培养法灵敏度可达1ng／ml，鸡胚背根神经节培养法需30ng／ml的浓度梯度才能在神经节上有所反应。结论：此实验样品为具有较高生物活性的高纯度NGF多肽。

Characterization of a new bradykinin-potentiating peptide (TmF) from Trimeresurus mucrosquamatus

A novel bradykinin-potentiating peptide (BPP), designated as TmF, has been purified to homogeneity from the venom of Trimeresurus mucrosquamatus by 70% cold methanol extraction, Sephadex G-15 gel filtration and reverse-phase high performance liquid chromatography (RP-HPLC). The amino acid sequence of TmF was determined to be pGlu-Gly-Arg-Pro-Leu-Gly-Pro-Pro-Ile-Pro-Pro (pGlu denotes pyroglutamic acid), which shared high homology with other BPPs. The molecular mass of TmF was 1.1107 kD as determinated by electrospray ionization-mass spectrometry (ESI-MS), which was in accordance with the calculated value of 1.1106 kD. The potentiating "unit" of TmF to bradykinin-induced (BK-induced) contraction on the guinea-pig ileum in vitro was (1.13 +/- 0.3) unit (mg/L), and TmF (5.0 x 10(-4) mg/kg) increased the pressure-lowering-effect of bradykinin (5.0 x 10(-5) mg/kg) with approximate descent value of (14 +/- 2) mmHg. In addition, TmF inhibited the conversion of angiotensin I to angiotensin 11, 2 x 10(-3) mg of TmF caused 50% inhibition (IC50) of angiotensin-converting enzyme (ACE) hydrolyzing activity to bradykinin.

无指盘臭蛙皮肤抗感染多肽组学研究

在过去的一个多世纪里，两栖类动物皮肤分泌液作为它们的第一道防御屏障引起了研究者们极大的兴趣，同时也开展了相关的许对研究，到目前为止，已从中分离鉴定出了百余种的活性物质。无指盘臭蛙是我国的一种特有两栖动物，初步的活性检测发现，无指盘臭蛙皮肤分泌液具有很强的抗菌，溶血以及蛋白酶抑制剂活性。 在本论文中，我们利用多肽组学与基因组学的方法对无指盘臭蛙皮肤的抗感染多肽组进行了研究。 通过三步分离纯化过程：一步Sephadex G-50分子筛和两步反相高压液相（RP-HPLC）的方法，从无指盘臭蛙皮肤分泌液中分离纯化得到了21条新的抗菌肽，它们分别属于17个不同的抗菌肽家族，其中8个分别属于已知的5个抗菌肽家族，它们是：Brevinin-1E(2个)、Brevinin-2E（1个）、Esculentin-1（1个）、Esculentin-2（1个）和Nigrocin（3个）抗菌肽家族。另外的13个抗菌肽与已发现的抗菌肽表现出较低的相似性，我们将它们归类到12种新的抗菌肽家族，它们是：Odorranain-A (1个)、Odorranain-B(1个)、 Odorranain-C(1个)、 Odorranain-G (1个)、Odorranain-H (2个)、 Odorranain-J (1个)、Odorranain-L (1个)、Odorranain-M (1个)、 Odorranain-N (1个)、 Odorranain-O (1个)、Odorranain-Q(1个)、 Odorranain-T(1个)。 从单个无指盘臭蛙皮肤里面，我们克隆得到了372条抗菌肽序列，它们编码107条新的抗菌肽，这一发现使得目前发现的两栖类抗菌肽的数目几乎增加了1倍。这也是目前发现的抗菌肽最为丰富的物种。这107条抗菌肽分别属于30个不同的抗菌肽家族，其中有24个为新的抗菌肽家族。这些抗菌肽的多样性可能是通过点突变、碱基的插入或删除、结构域的穿梭以及拼接等多种机制形成的。这些抗菌肽多样性的形成可能与无指盘臭蛙生活环境中微生物的组成有关。30个家族抗菌肽前体序列的SPD区域（包括信号肽和前导肽序列，Signal and Propiece Domain, SPD）非常保守，表明它们可能起源于同一个祖先基因。对7个抗菌肽家族的非同义碱基替代率Dn与同义碱基替代率Ds进行检测发现，它们可能经受着不同选择压力的作用。无指盘臭蛙皮肤抗菌肽在二级结构和功能上都表现出丰富的多样性。在一个两栖类个体里面发现如此丰富的抗菌肽甚是让人惊讶。这一发现也使得我们不得不重新认识先天性免疫在两栖类动物防御系统中的重要性，对两栖类生态环境的分子基础以及那种认为一种两栖类只需要20-30种抗菌肽就足以抵御环境中的微生物的看法重新审视。我们的研究还显示：无指盘臭蛙抗菌肽之间还存在着协同效用。 我们对无指盘臭蛙皮肤抗菌肽的去极化作用进行了研究，发现所检测的7个抗菌肽都可使金黄色葡萄球菌发生去极化，但是它们使细菌发生去极化的能力不同。对12种抗菌肽的抗菌机制研究发现，它们通过多种不同的机制发挥作用：有些在细菌内形成片层样的囊泡状结构，有些导致细胞质壁的分离，有些在细菌的膜上形成穿孔，有些则导致了细菌染色质的固缩。 总之，这些研究为设计新型的抗菌肽提供了有用的参考资料。

基于光合色素的化学分类法在淡水藻类研究中的应用

采用反相高效液相色谱技术(RP-HPLC)系统研究了我国主要淡水藻类———蓝藻、绿藻、硅藻、甲藻、金藻、裸藻和隐藻等的光合色素,在8种纯培养藻类中共确定类胡萝卜素、叶绿素及其衍生物19种。分离到的主要标志性色素按洗脱时间分别为脱植基叶绿素a、19′-丁酰氧岩藻黄素、叶绿素c、脱镁叶绿素a、多甲藻素、甲基脱植基叶绿素a、岩藻黄素、新黄质、紫黄质、蓝藻叶黄素、硅甲藻黄素、硅藻黄质、叶黄素、玉米黄素、叶绿素b异构体、叶绿素b、叶绿素a异构体、叶绿素a和β-胡萝卜素;其中在纯培养的铜绿微囊藻中首次鉴定到19′-丁

金藻吞噬微囊藻产生的无毒变异株与产毒原始株的比较

分别从喂食三株原始产毒铜绿微囊藻Microcystis aeruginosa(AC、DS和PCC 7820)的金藻Poterioochromonassp.培养物中获得三株藻,以Nest PCR方法(引物对CC/CG和CH/CI)确定此三株藻均为微囊藻属藻株。HPLC测试结果显示这三株藻均不产生微囊藻毒素。显示Poterioochromonassp.具有将产毒微囊藻转化为无毒微囊藻的能力。比较产毒原始株与无毒变异株的生理特性发现,变异株的类胡萝卜素/叶绿素比值高于原始株;而光反应曲线结果表明,变异株的PSⅡ

六溴环十二烷异构体在鮰鱼体内的浓度分布与生物累积特征

研究了鮰鱼体内六溴环十二烷(HBCDs)异构体的浓度分布与生物累积特征。首先采用基质固相分散(MSPD)法,同位素稀释定量,高效液相色谱-电喷雾串联质谱(HPLC-ESI-MS/MS)检测技术,建立了渔业饲料和鱼体中α-HBCD、β-HBCD和γ-HBCD的分析方法。该法对α-HBCD、β-HBCD、γ-HBCD的回收率分别为80.7%~110.5%、80.1%~109.0%、86.9%~104.5%,其检出限分别为0.002、0.002、0.001 ng/g。采用所建立的方法对25个渔业饲料样品和30个

野生与豢养长江江豚血清氨基酸含量比较

应用高效液相色谱(HPLC)技术,首次测定了湖北石首长江天鹅州白豚自然保护区野生长江江豚(Neopho-caena phocaenoides asiaeorientalis)和中国科学院水生生物研究所白豚馆人工饲养的长江江豚血清中17种氨基酸的含量。结果表明,除了脯氨酸Pro、蛋氨酸Met和组氨酸His外,人工饲养江豚血清中其余14种氨基酸(天门冬氨酸Asp、谷氨酸Glu、丝氨酸Ser、精氨酸Arg、甘氨酸Gly、苏氨酸Thr、丙氨酸Ala、异亮氨酸Ile、亮氨酸Leu、苯丙氨酸Phe、缬氨酸Val、赖氨

微囊藻毒素[Dha~7]MCRR的制备及鉴定

以野外收集的水华蓝藻为原料,经过75%甲醇溶液浸提,快速色谱分离和半制备色谱纯化,从滇池水华蓝藻中分离纯化出1种微囊藻毒素变体.电喷雾质谱、紫外分光光度计和HPLC检测结果表明,所得毒素为[Dha7]MCRR,是MCRR的1种去甲基化变体,其纯度大于95%.该毒素的分子组成为环(Ala-Arg-MeAsp-Arg-Adda-Glu-Dha),分子量为1 023,其紫外扫描光谱(200~300 nm)在239 nm处有特征吸收.[Dha7]MCRR在滇池水华蓝藻中普遍存在,有时会成为MC的主要种类.

微囊藻毒素RR的制备及鉴定

以野外收集的水华蓝藻为原料,建立了以75%甲醇溶液提取、快速色谱和半制备色谱分离为主要步骤的微囊藻毒素分离纯化方法,并用HPLC、分光光度计和电喷雾质谱对所得毒素的纯度和结构进行了鉴定.结果表明,所得毒素为MCRR,纯度大于95%,其紫外吸收光谱在239nm处有特征吸收,分子组成为环(Ala-Arg-MeAsp-Arg-Adda-Glu-Mdha),分子量为1037.