具有中等毒性的马氏钳蝎神经毒素的纯化和初步晶体学…

运用柱层析技术对产自淅川和常德的马氏钳蝎毒素进行分离纯化,得到８种哺乳动物神经毒素。运用制备型等电聚焦电泳技术,对常德样品中具有中等毒性的蝎神经毒素进一步纯化,获得了高纯度样品。两个产地的蝎毒素ＢｍＫ５均已经成功地获得了大晶体。空间群均为Ｐ２１２１２１,晶胞参数分别为：ａ＝３８．４６埃,ｂ＝３７．２８埃,ｃ＝３６．９７埃;ａ＝３８．４４埃,ｂ＝３７．５５埃,ｃ＝３６．８３埃。对两个产地的晶体分别收     

一种东亚钳蝎碱性神经毒素的纯化和初步晶体学研究

经ＳｅｐｈａｄｅｘＧ－５０和ＳＰ－ＳｅｐｈａｄｅｘＣ－２５两次柱层析,从河南淅川马氏钳蝎毒素中分得一种碱性神经毒素ＢｍＫＭＩ８．等电聚焦和ＳＤＳ电泳显示单一组分,其ｐＩ为９．１,Ｍｒ为７１００．毒性测试结果表明,该组分对小白鼠有较强的毒性,对昆虫也有一定的毒性,已获得该毒素的两种晶型的大单晶,并测定其空间群为Ｐ２＿１２＿１２＿１,晶胞参数为：ＢｍＫＭＩ８－Ａ：ａ＝３６．７,ｂ＝２６．６,ｃ＝５２．０,ＢｍＫＭＩ８－Ｂ：ａ＝３６．６４Ａ,ｂ＝３７．３１,ｃ＝３７．９５,已收集了ＢｍＫＭＩ８－Ｂ分辨率为１．７４的Ｘ射线单晶衍射数据。     

一种东亚钳蝎碱性神经毒素的纯化和初步晶体学研究

经ＳｅｐｈａｄｅｘＧ－５０和ＳＰ－ＳｅｐｈａｄｅｘＣ－２５两次柱层析,从河南淅川马氏钳蝎毒素中分得一种碱性神经毒素ＢｍＫＭＩ８。等电聚聚焦和ＳＤＳ电泳显示单一组分,其ＰＩ为９．１,Ｍｒ为７１００,毒性测试结果表明,该组分对小白鼠有较强的毒性,对昆虫也有一定的毒性。已获得该毒素的两种晶全型的大单晶,并测定其空间群为Ｐ２１２１２１,晶胞参数为：ＢｍＫＭＩ８－Ａ：ａ＝３６．７Ａ,ｂ＝２６．６Ａ,ｃ＝５２     

东亚钳蝎神经毒素在大肠杆菌中的表达

以山西风陵渡东亚钳蝎（ＢｕｔｈｕｓｍａｒｔｅｎｓｉＫａｒｓｃｈ）的尾腺总ＲＮＡ为模板,根据已知的蝎神经毒素保守氨基酸序列设计引物,利用ＰＣＲ技术,扩增并克隆了两个蝎神经毒素基因．序列分析表明,由两个基因导出的氨基酸序列（ＢｍＫＭｍ１和ＢｍＫＭｍ２）与已知的蝎神经毒素ＢｍＫⅠ、ＢｍＫⅡ、ＢｍＫⅢ、ＢｍＫＭ１、ＢｍＫＭ９有很高的同源性．将ＢｍＫＭｍ２基因重组到大肠杆菌分泌型表达载体ｐＥｘＳｅｃ１中进行表达．ＳＤＳ－ＰＡＧＥ证明表达产物被分泌到细胞周间质及培养液中．经ＩｇＧ－Ｓｅｐｈａｒｏｓｅ纯化后的蛋白质注射小白鼠表明表达产物有生物学活性     

仲彬草属5种植物的核型研究

本文对我国西部高原仲彬草属Ｋｅｎｇｙｉｌｉａ５种植物的核型进行了分析。它们的染色体数目均为２ｎ＝４２,六倍体。核型是：糙毛鹅观草Ｋ．ｈｉｒｓｕｔａ,２ｎ＝６ｘ＝４２＝３６６＋６ｓｍ;青海鹅观草Ｋ．ｋｏｋｏｎｏｒｉｃａ,２ｎ＝６ｘ＝４２＝３６ｍ＋６ｓｍ：黑药鹅观草Ｋ．ｍｅｌａｎｔｈｅｒａ,２ｎ＝６ｘ＝４２＝３８ｍ＋４ｓｍ;硬秆鹅观草Ｋ．ｒｉｇｉｄｕｌａ,２ｎ＝６ｘ＝４２＝３８ｍ＋４ｓｍ;窄颖鹅观草Ｋ．ｓｔｅｎａｃｈｙｒａ,２ｎ＝６ｘ＝４２＝３８ｍ＋４ｓｍ。它们的核型属于１Ｂ或２Ｂ型。染色体中均未发现随体。     

山东四种草本植物的核型研究

本文对山东４种草本植物进行了染色体研究。结果表明：阿尔泰狗哇花（Ｈｅｔｅｒｏｐａｐｐｕｓａｌ ｔａｉｃｕｓ（Ｗｉｌｄ）Ｎａｖｏｐｏｋｒ）的染色体数目为２ｎ＝３６,核型公式为Ｋ（２ｎ）＝３６＝３６ｍ,核型“１Ａ”型;求米草（Ｏｐｌｉｓｍｅｎｕｓｕｎｄｕｌａｔｉｆｏｌｉｕｓ（Ａｒｄｕｉｎｏ）ＲｏｅｍｅｔＳｃｈｕｌｔ）的染色体数目为２ｎ＝１２,核型公式为Ｋ（２ｎ）＝１２＝８ｍ＋４ｓｍ,核型“２Ａ”型;红秋葵（Ｈｉｂｉｓｃｕｓｃｏｃｉｎｅｕｓ（Ｍｅｄｉｃ）Ｗａｌｔ）的染色体数目为２ｎ＝３８,核型公式为Ｋ（２ｎ）＝３８＝１４ｍ＋２２ｓｍ＋２ｓｔ,核型“２Ｂ”型;蟋蟀草（Ｅｌｅｕｓｉｎｅｉｎｄｉｃａ（Ｌ）Ｇａｅｒｔｎ）的染色体数目为２ｎ＝１８,核型公式为ｋ（２ｎ）＝１８＝１６ｍ＋２ｓｍ,核型“２Ａ”型。     

B链氨端去－肽（B1）羧端去五肽（B26—30）猪胰岛素的初步晶体学研究

应用悬滴气相扩散法在含６％氯化纳和１２．５％丙酮的柠檬酸缓冲体系中,获得可供Ｘ射线结构分析用的Ｂ链氨端去一肽（Ｂ１）羧端去五肽（Ｂ２６—３０）猪胰岛素（ＤｅｓＢ１－ＤＰＩ）单晶体。晶体属四方晶系,空间群为Ｐ４１２２或Ｐ４３２２,晶胞参数为：ａ＝ｂ＝３６．０Ａ,ｃ＝１２０．０Ａ,ａ＝β＝γ＝９０°。单位晶胞中每个结晶学不对称单位含有２个ＤｅｓＢ１—ＤＰＩ分子。     

一种强毒性中华马氏钳蝎哺乳动物神经毒素新晶型的初步晶体学研究

经ＳｅｐｈａｄｅｘＧ－５０和Ｓｐ－ＳｅｐｈａｄｅｘＣ－２５两次柱层析,从常德马氏钳蝎毒素中分离得到一种强毒性的哺乳动物神经毒（Ｂｍｋｌ）,等电聚焦及ＳＤＳ－电泳显示它为单一组份,其ｐＩ为９．４４,ＭＷ为７．１ＫＤ．毒性试验结果表明,该组份对小白鼠的最小致死刘量为０．５μｇ／ｇ小白鼠,对昆虫及甲壳动物也有毒性．已获得该毒素的一种新晶型的大晶体。其空间群为Ｐ２１２１２,晶胞参数为：α＝８３．４６Ａ,ｂ＝４０．３６Ａ,ｃ＝２４．００Ａ,单位晶胞体积为８０８４２．６９Ａ,一个不对称单位含１个分子,已收集了分辨率为１．７５Ａ的数据．     

B链氨端去－肽（B1）羧端去五肽（B26—30）猪胰岛素的初步晶体学研究

应用悬滴气相扩散法在含６％氯化钠和１２．５％丙酮的柠檬酸缓冲体系中,获得可供Ｘ射线结构分析用的Ｂ链氨端去－肽（Ｂ１）羧端去五肽（Ｂ２６－３０）猪胰岛素单晶体。晶体属四方晶系,空间群为Ｐ４１２２或Ｐ４３２２,晶胞参数为：ａ＝ｂ＝３６．０Ａ,ｃ＝１２０．０Ａ,α＝β＝γ＝９０度。单位晶胞中每个结晶学不对称单位含有２个ＤｅｓＢ１－ＤＰＩ分子。     

七种药用植物的染色体研究

对山东７种药用植物的染色体进行了研究。结果表明：田旋花（ＣｏｎｖｏｌｖｕｌｕｓａｒｖｅｎｓｉｓＬ）的染色体数目为２ｎ＝７８;蜜柑草（ＰｈｙｌａｎｔｈｕｓｍａｔｓｕｍｕｒａｅＨａｖａｔａ）的染色体数目为ｎ＝８８;挂红灯（ＰｈｙｓａｌｉｓａｌｋｅｋｅｎｇｉＬｖａｒｆｒａｎｃｈｅｔｉ（Ｍａｓｔ）Ｍａｋｉｎｏ）的染色体数目为２ｎ＝２４,核型公式为Ｋ（２ｎ）＝２４＝２ｍ＋１８ｓｍ＋２ｓｔ＋２ｓｔ（ｓａｔ）,核型“２Ａ”型;无剌曼陀罗（ＤａｔｕｒａｓｔｒａｍｏｎｉｕｍＬｖａｒｉｎｅｒｍｉｓ（Ｊａｃｑ）ＳｃｈｉｎｚｅｔＴｈｅｌ）的染色体数目为２ｎ＝２４,核型公式为Ｋ（２ｎ）＝２４＝２０ｍ＋４ｓｍ,核型“１Ｂ”型;决明（ＣａｓｉａｔｏｒａＬ）的染色体数目为２ｎ＝２６,核型公式为Ｋ（２ｎ）＝２６＝２４ｍ＋２ｓｍ,核型“１Ａ”型;荔枝草（ＳａｌｖｉａｐｌｅｂｅｉａＲＢｒ）的染色体数目为２ｎ＝１６,核型公式为Ｋ（２ｎ）＝１６＝６ｍ＋１０ｓｍ,核型“２Ａ”型;车前（ＰｌａｎｔａｇｏａｓｉａｔｉｃａＬ）的染色体数目为２ｎ＝３６,核型公式为Ｋ（２ｎ）＝３６＝３２ｍ＋４ｓｍ,核型“１Ａ”型。     

Crystal structure determination of an acidic neurotoxin (BmK M8) from scorpion Buthm martensii Karsch at 0.25nm resolution

The crystal structure of an acidic neurotoxin, BmK M8, from Chinese scorpion Buthus martensii Karsch was determined at 0.25 nm resolution. The X-ray diffraction data of BmK M8 crystals at 0.25nm resolution were collected on a Siemens area detector. Using molecular replacement method with a basic scorpion toxin AaH II in a search model, the cross-rotation function, PC-refinement and translation function were calculated by X-PLOR program package. The correct orientation and position of BmK M8 molecule in crystal were determined in a resolution range of 1.5 - 0.35nm, The oystallographic refinement was further performed by stereo-chemical restrict least-square technique, followed by simulated annealing, slow-cooling protocols. The final crystallographic R-factor at 0.8-0.25 nm is 0.171. The standard deviations of bond length and bond angle from ideality are 0.001 7nm and 2.24° , respectively. The final model of BmK M8 structure is composed of a dense core of secondary structure elements by a stretch of α-     

Crystallization and preliminary X-ray analysis of botulinum neurotoxin type A.

Botulinum neurotoxin serotype A was isolated from liquid culture of Clostridium botulinum. The pure Mr approximately 150,000 neurotoxin, composed of Mr approximately 50,000 light and Mr approximately 100,000 heavy chains, has been crystallized in three different crystal morphologies; all three have the same crystal form. The most suitable crystal form for X-ray analysis are bipyrimidal and crystallize in the hexagonal space group P3(1)21 (or P3(2)21) with one dimer per asymmetric unit. The unit cell dimensions are a = b = 170.5 A, c = 161.7 A. The crystals diffract to 3 A resolution.     

不同产地中华马氏钳蝎神经毒素的分离纯化和部分性质比较研究

经Ｓｅｐｈａｄｅｘ Ｇ－５０,Ｓｐ－Ｓｅｐｈａｄｅｘ Ｃ－２５两次柱层析,从没产地的东亚马氏钳歇粗毒中分别得到了一组碱性哺乳动物神经素和一种甲壳类神经毒素,对它们进行的等电点、分子量、动物毒性等部分性质的研究与比较结果表明,淅川、常德与益都产的蝎毒无论在柱层析行为上,还是在等电点、分子量、各组分的毒性大顺序及某些对应组分的结晶行为上有很大相似性,仅存在略微的差异。     

Crystal structure determination of a neutral neurotoxin BmK M4 from Buthus martensii Karsch at 0.20 nm

BmK M4 is a neutral neurotoxin in the BmK toxin series.It is medially toxic and belongs to group III α-toxins.The purified sample was crystallized in rhombic space group P61.Using an X-ray diffraction technique,the crystal structure of BmK M4 was revealed by molecular replacement at 0.20 nm resolution.The model was refined.The final crystallographic R factor was 0.142 and the free R factor was 0.173.The root mean square deviation is 0.001 5 nm for the bond length and 1.753°for the bond angles.64 water molecules were added to the asymmetric unit.The refined structure showed an unusual non-prolyl cis peptide bond at residue 10.The structure was compared with group II α-toxin BmK M8 (an acidic,weak toxin).The potential structural implications of the cis peptide bond were discussed.     

Exploring the obscure profiles of pharmacological binding sites on voltage-gated sodium channels by BmK neurotoxins

Diverse subtypes of voltage-gated sodium channels (VGSCs) have been found throughout tissues of the brain, muscles and the heart. Neurotoxins extracted from the venom of the Asian scorpion Buthus martensi Karsch (BmK) act as sodium channel-specific modulators and have therefore been widely used to study VGSCs. α-type neurotoxins, named BmK I, BmK αIV and BmK abT, bind to receptor site-3 on VGSCs and can strongly prolong the inactivation phase of VGSCs. In contrast, β-type neurotoxins, named BmK AS, BmK AS-1, BmK IT and BmK IT2, occupy receptor site-4 on VGSCs and can suppress peak currents and hyperpolarize the activation kinetics of sodium channels. Accumulating evidence from binding assays of scorpion neurotoxins on VGSCs, however, indicate that pharmacological sensitivity of VGSC subtypes to different modulators is much more complex than that suggested by the simple α-type and β-type neurotoxin distinction. Exploring the mechanisms of possible dynamic interactions between site 3-/4-specific modulators and region- and/or species-specific subtypes of VGSCs would therefore greatly expand our understanding of the physiological and pharmacological properties of diverse VGSCs. In this review, we discuss the pharmacological and structural diversity of VGSCs as revealed by studies exploring the binding properties and cross-competitive binding of site 3- or site 4-specific modulators in VGSC subtypes in synaptosomes from distinct tissues of diverse species.     

Chinese-scorpion (Buthus martensi Karsch) toxin BmK alphaIV, a novel modulator of sodium channels: from genomic organization to functional analysis

In the present study, BmK alphaIV, a novel modulator of sodium channels, was cloned from venomous glands of the Chinese scorpion (Buthus martensi Karsch) and expressed successfully in Escherichia coli. The BmK alphaIV gene is composed of two exons separated by a 503 bp intron. The mature polypeptide contains 66 amino acids. BmK alphaIV has potent toxicity in mice and cockroaches. Surface-plasmon-resonance analysis found that BmK alphaIV could bind to both rat cerebrocortical synaptosomes and cockroach neuronal membranes, and shared similar binding sites on sodium channels with classical AaH II (alpha-mammal neurotoxin from the scorpion Androctonus australis Hector), BmK AS (beta-like neurotoxin), BmK IT2 (the depressant insect-selective neurotoxin) and BmK abT (transitional neurotoxin), but not with BmK I (alpha-like neurotoxin). Two-electrode voltage clamp recordings on rNav1.2 channels expressed in Xenopus laevis oocytes revealed that BmK alphaIV increased the peak amplitude and prolonged the inactivation phase of Na+ currents. The structural and pharmacological properties compared with those of other scorpion alpha-toxins suggests that BmK alphaIV represents a novel subgroup or functional hybrid of alpha-toxins and might be an evolutionary intermediate neurotoxin for alpha-toxins.     

Purification,crystallization and initial structural solution of a new alpha-like toxin with cardiac toxicity from scorpion Buthus martensii Karsch

An alpha-like toxin named BmK M7 active on both mammals and insects has been purified from the venom of scorpion Buthus martensii Karsch (BmK) recently. The electrophysiological experiments showed that M7 can bind to human cardiac Na+-channel and modify its normal properties, hence can be considered as a cardiotoxin. Single crystals of M7 have been obtained by hanging-drop vapor diffusion method using ammonium sulfate as precipitant in Tris-HCl buffer at pH 8.5. A data set to 1.40 A resolution was collected using synchrotron radiation and CCD detector in Photon Factory in Japan. Data analysis showed that the crystals belonged to space group P3(1)21/P3(1)21, with cell dimensions a=b=32.76 A, c=176.82 A. Assuming two molecules per asymmetric unit, the Vm value is 1.92 A3/Da. The initial structural analysis was carried out by molecular replacement, which showed the correct space group (P3(1)21), and the orientations and positions of the two molecules in the asymmetric unit.     

Crystal structure determination of a neutral neurotoxin BmK M4 fromButhus martensii Karsch at 0.20 nm

BmK M4 is a neutral neurotoxin in the BmK toxin series. It is medially toxic and belongs to group III cc-toxins. The purified sample was crystallized in rhombic space group P6 Using an X-ray diffraction technique, the crystal structure of BmK M4 was revealed by molecular replacement at 0.20 nm resolution. The model was refined. The final crystallographic R factor was 0.142 and the free R factor was 0.173. The root mean square deviation is 0.001 5 nm for the bond length and 1.753° for the bond angles. 64 water molecules were added to the asymmetric unit. The refined structure showed an unusual non-prolyl cis peptide bond at residue 10. The structure was compared with group II a-toxin BmK M8 (an acidic, weak toxin). The potential structural implications of the cis peptide bond were discussed.     

Structural mechanism governing cis and trans isomeric states and an intramolecular switch for cis/trans isomerization of a non-proline peptide bond observed in crystal structures of scorpion toxins

Non-proline cis peptide bonds have been observed in numerous protein crystal structures even though the energetic barrier to this conformation is significant and no non-prolyl-cis/trans-isomerase has been identified to date. While some external factors, such as metal binding or co-factor interaction, have been identified that appear to induce cis/trans isomerization of non-proline peptide bonds, the intrinsic structural basis for their existence and the mechanism governing cis/trans isomerization in proteins remains poorly understood. Here, we report the crystal structure of a newly isolated neurotoxin, the scorpion alpha-like toxin Buthus martensii Karsch (BmK) M7, at 1.4A resolution. BmK M7 crystallizes as a dimer in which the identical non-proline peptide bond between residues 9 and 10 exists either in the cis conformation or as a mixture of cis and trans conformations in either monomer. We also determined the crystal structures of several mutants of BmK M1, a representative scorpion alpha-like toxin that contains an identical non-proline cis peptide bond as that observed in BmK M7, in which residues within or neighboring the cis peptide bond were altered. Substitution of an aspartic acid residue for lysine at residue 8 in the BmK M1 (K8D) mutant converted the cis form of the non-proline peptide bond 9-10 into the trans form, revealing an intramolecular switch for cis-to-trans isomerization. Cis/trans interconversion of the switch residue at position 8 appears to be sequence-dependent as the peptide bond between residues 9 and 10 retains its wild-type cis conformation in the BmK M1 (K8Q) mutant structure. The structural interconversion of the isomeric states of the BmK M1 non-proline cis peptide bond may relate to the conversion of the scorpion alpha-toxins subgroups.