粗毛栓菌胞外锰过氧化物酶的纯化及性质

培养于麦草粉上的白腐担子菌粗毛栓菌分泌胞外木质纤维素降解酶(纤维素酶、木聚糖酶、漆酶、锰过氧化物酶和木质素过氧化物酶)。经过超滤、盐析、离子交换层析、凝胶过滤和活性聚丙烯酰胺凝胶电泳等步骤,获得了初步纯化的锰过氧化物酶组分。利用变性聚丙烯酰胺凝胶电泳和等电点聚焦技术所测定的锰过氧化物酶的相对分子质量和等电点分别为35.7 ku和pI 2.8。研究结果表明,所纯化的锰过氧化物酶在407nm处具有最大光吸收峰,该酶最适作用pH值和温度分别为pH 5.3和35℃。     

黑曲霉A3木聚糖酶酶学性质研究

黑曲霉A3(AspergillusnigerA3)的固体培养物浸出液,经过多步分离纯化后,获得三个组份的木聚糖酶,称为xⅠ、xⅡ和xⅢ.经7%凝胶浓度的盘状电泳分析均为单一组份.经等电聚焦电泳测xⅠ、xⅡ和xⅢ的等电点分别为6.8、5.5和6.1.SDS-PAGE测得亚基分子量(Da)分别为xⅠ,42000;xⅡ,20000;xⅢ,31000.三个酶组份的最适反应温度分别为xⅠ,40℃;xⅡ,50℃;xⅢ,50℃.最适反应pHxⅠ,3.5;xⅡ,4.5;xⅢ,5.0.保温一个小时后,酶的半失活温度分别为xⅠ,55.6℃;xⅡ,54.8℃;xⅢ,46.6℃.金属离子Ag+、Hg2+、Ni2+和脲对不同的酶组份具有一定的影响.     

棘孢曲霉SML22木聚糖酶系主要组分的纯化与性

经超滤浓缩、分子筛色谱、阴离子和阳离子交换层析,由棘孢曲霉发酵液最终分离得到4个电泳纯的木聚糖酶主要组分Xy-1、Xy-2、Xy-3和Xy-4。通过SDS聚丙烯酰胺凝胶电泳测得各组分的分子量分别是92.13、32.40、42.40和27.03 kD。实验证明这些酶组分均属于酸性木聚糖酶,Xy-1、Xy-2、Xy-3和Xy-4的最适反应pH分别为5.0、4.0、4.6 和3～3.5。各酶组分在酸性条件下较稳定,碱性条件下酶活丧失较快。Xy-1及Xy-2的最适反应温度在75℃,在50℃以下比较稳定;Xy-3及Xy-4最适反应温度为55℃,在40℃以下比较稳定。通过对各酶组分米氏常数的测定可知,Xy-1及Xy-2对底物桦木木聚糖的Km值分别为0.36%和0.26%,Xy-3及Xy-4的Km值为2.46%和13.9%。4种组分的Vmax分别为4.01μmol/min/mg、8.81μmol/min/mg、81.97μmol/min/mg、4.71μmol/min/mg。Cu2+、Ag+对各组分都有较强的抑制作用, Mg2+、Ba2+、Ca2+能促进Xy-3的木聚糖酶活,Ca2+也可大幅度促进Xy-4的木聚糖酶活性。     

绿色木霉木聚糖酶的纯化和性质

绿色木霉木聚糖酶经分离纯化后,获得三个组分木聚糖酶,称为XⅠ,XⅡ和XⅢ,它们最反应温度分别为60℃、60℃、50℃,pH分别为5．5、5．0、0、4．5,pⅠ分别为XⅠ3．8,XⅡ3．4,XⅢ3．6。半失活温度分别为XⅠ37℃,XⅡ44℃,XⅢ40℃。     

黑曲霉A3木聚糖酶酶学性质研究*

黑曲霉A3（AspergillusnigerA3）的固体培养物浸出液,经过多步分离纯化后,获得三个组份的木聚糖酶,称为xⅠ、xⅡ和xⅢ。经7％凝胶浓度的盘状电泳分析均为单一组份。经等电聚焦电泳测xⅠ、xⅡ和xⅢ的等电点分别为6.8、5．5和6.1。SDS－PAGE测得亚基分子量（Da）分别为xⅠ,42000;xⅡ,20000;xⅢ,3000。三个酶组份的最适反应温度分别为xⅠ,40℃i;xⅡ,50℃;xⅢ,50℃。最适反应pHxⅠ,3．5;xⅢ,4．5;xⅢ,5．0。保温一个小时后,酶的半失活温度分别为xⅠ,55.6℃;xⅡ,54.8℃;xⅢ,46.6℃。金属离子Ag+、Hg2+、Ni2+和脲对不同的酶组份具有一定的影响。     

耐冷皮壳正青霉一种木聚糖酶的纯化与性质研究

研究了耐冷皮壳正青霉Eupenicillium crustaceum一种木聚糖酶的纯化和酶学性质。采用硫酸铵沉淀和阴离子交换层析的方法,从耐冷皮壳正青霉液体发酵液中分离纯化出一种亚基分子量35kDa的木聚糖酶。酶学性质研究表明,酶的最适pH值为5.5,在pH4.5-6.5范围内具有较高的催化活性。最适温度为50℃,20℃下酶活为最高酶活的40%。Ag+和Fe2+大幅度提高木聚糖酶的酶活,而Mn2+和Hg2+强烈抑制木聚糖酶的活性。同时,该木聚糖酶具有严格的底物特异性。     

黑曲霉产木聚糖酶的分离纯化与鉴定研究

木聚糖酶的分离纯化是对其进行酶学研究和分子改良研究的基础。利用实验室选育的黑曲霉菌株Aspergillus niger SM24/a进行木聚糖酶发酵,粗酶液经过(NH_4)_2SO_4分级沉淀Bio-Gel P6除盐、UNO sphere Q阴离子交换和Enrich SEC70凝胶色谱层析四个步骤的分离纯化,成功获得了3种木聚糖酶蛋白定义为X-Ⅰ、X-Ⅱ和X-Ⅲ。随着纯化步骤的增加,各组分酶比活力得到显著提高,其数值分别为37.41、34.56和53.96 U/mg,纯化倍数分别为3.96、3.66和5.72。经质谱分析和蛋白氨基酸序列比对,初步认定X-Ⅰ属于糖基水解酶第十家族内切-β-1,4-木聚糖酶,X-Ⅱ和X-Ⅲ均属于糖基水解酶第十一家族木聚糖酶。     

M-26碱性木聚糖酶的分离纯化及酶学性质研究

从Bacillus pumilus M-26发酵液中分离纯化碱性木聚糖酶,进行酶学性质研究,同时制备工业用碱性木聚糖酶制剂。首先将M-26发酵液进行硫酸铵盐析,制备工业用碱性木聚糖酶干品;然后进行sephadexG-25层析脱盐和cellulose DE-52层析得以纯化。硫酸铵的饱和度50%,酶制剂的酶活可达9 000 IU/g,收率为85%;分离纯化使酶的比活为126.32 IU/mg蛋白,纯化倍数为19.89,酶的回收率12.83%;分子量约为20 ku;M-26碱性木聚糖酶的最适温度和pH分别是55℃和pH 8.0,具有一定的耐碱性;该酶无纤维素酶活性,Fe2＋对其有激活作用;Mn2＋、Zn2＋、Fe3＋、Cu2＋对其具有抑制作用。短小芽胞杆菌M-26碱性木聚糖酶具有纸浆生物漂白应用前景。     

黑曲霉A3木聚糖酶酶学性质研究

黑曲霉Ａ３（Ａｓｐｅｒｇｉｌｌｕｓ ｎｉｇｅｒ Ａ３）的固体培养物浸出液,经过多步分离纯化后,获得三个组份的木聚糖酶,称为ｘⅠ、ｘⅡ和ｘⅢ。经７％凝胶浓度的盘状电泳分析均为单一组份。经等电聚焦电泳测ｘⅠ、ｘⅡ和ｘⅢ。的等电点分别为６．８、５．５和６．１。ＳＤＳ－ＰＡＧＥ测得亚基分子量（Ｄａ）分别为ｘⅠ,４２０００;ｘⅡ,２００００;ｘⅢ,３１０００。三个酶组份的最适反应温度分别为ｘⅠ,４０℃;ｘⅡ     

棘孢曲霉SM-L22木聚糖酶系主要组分的纯化与性质

经超滤浓缩、分子筛色谱、阴离子和阳离子交换层析 ,由棘孢曲霉发酵液最终分离得到 4个电泳纯的木聚糖酶主要组分Xy 1、Xy 2、Xy 3和Xy 4。通过SDS 聚丙烯酰胺凝胶电泳测得各组分的分子量分别是 92 1 3、32 4 0、4 2 4 0和 2 7 0 3kD。实验证明这些酶组分均属于酸性木聚糖酶 ,Xy 1、Xy 2、Xy 3和Xy 4的最适反应pH分别为 5 0、4 0、4 6和 3～ 3 5。各酶组分在酸性条件下较稳定 ,碱性条件下酶活丧失较快。Xy 1及Xy 2的最适反应温度在75℃ ,在 5 0℃以下比较稳定 ;Xy 3及Xy 4最适反应温度为 5 5℃ ,在 4 0℃以下比较稳定。通过对各酶组分米氏常数的测定可知 ,Xy 1及Xy 2对底物桦木木聚糖的Km 值分别为 0 36 %和 0 2 6 % ,Xy 3及Xy 4的Km 值为 2 4 6 %和1 3 9%。 4种组分的Vmax 分别为 4 0 1 μmol min mg、8 81 μmol min mg、81 97μmol min mg、4 71 μmol min mg。Cu2 、Ag 对各组分都有较强的抑制作用 ,Mg2 、Ba2 、Ca2 能促进Xy 3的木聚糖酶活 ,Ca2 也可大幅度促进Xy 4的木聚糖酶活性。     

培养料配方对姬松茸子实体产量和氨基酸、有害物含量的影响

采用3种培养料配方,研究其对姬松茸(N2)产量和氨基酸含量有害物含量的影响。结果表明:姬松茸子实体中镉含量比培养料中高184～215倍,姬松茸有富集镉的特性。配方1、配方2、配方3子实体镉含量分别为13,10,9.6mg/kg,产量分别为9.5,9.4,8.8kg/m2,氨基酸总量分别为27.59%,25.80%,20.58%。配方2子实体中镉含量显著低于配方1,其产量、氨基酸总量与配方1相近;配方3的产量、氨基酸总量最低,与配方1、配方2差异显著,表明采用KH2PO4代换过磷酸钙,可以降低子实体镉含量,而不宜用化学氮代换牛粪;配方1子实体砷含量最高,与配方2、配方3差异显著。3种配方子实体中六六六、滴滴涕、敌敌畏、四环素等有害物含量基本相同。     

An Apomictic Autotriploid Line TAR Identified in Oryza sativa

Since apomixis has a close correlation with polyploidy and sterility, a number of autotriploids with no sexual reproductivity were induced and apomictic germplasm were screened in Oryza sativa L. As a result, an autotriploid line, named TAR, was cytoembryologically identified which possessed apomictic property, with an average seed-set rate of 10% per panicle. Karyotype analysis proved that all the progeny seeds of TAR carried 36 chromosomes in the generations tested. Priliminary cytological observations revealed that all the ovaries of TAR had embryo sac differentiation, 33% of which developed into normal megagametophyte, 9% with previous embryogenesis prior to anthesis, and about 58% differentiated abnormally, i.e. disordered polarization, absent female generative unit and more than 2 polar nuclei. In TAR, the frequencies of chromosome configuration of 12 Ⅲ, 11 Ⅱ + 1 Ⅱ +1 Ⅰ. L0Ⅲ +2Ⅱ +2 Ⅰ, 9Ⅲ+3Ⅱ +3 Ⅰ, 8Ⅲ+4Ⅱ +4 Ⅰ and 7Ⅲ+5 Ⅱ +5 Ⅰ were ll%, 17%, 15%, 26%, 20% and 11% respectively at metaphase Ⅰ . While in the check line T-15 of autotriploid only 7 % of the ovaries observed had embryo sac development, and the progenies of this triploid line were aneuploids with chromosome number of 25～27. In T-15, the frequencies of chromosome configuration of 12 Ⅲ, 11Ⅲ +1 Ⅱ +1 Ⅰ, 10 Ⅲ +2 Ⅱ +2 Ⅰ , 9Ⅲ+3 Ⅱ +3 Ⅰ and 8 Ⅲ+4 Ⅱ +4 Ⅰ were 24%, 16%, 36%, 17% and 7% respectively at metaphse Ⅰ . The above observations indicated that some megaspore mother cell in TAR might undergo apomeiosis and where it gave rise to unreduced embryo sac, the unreduced eggs or synergids developed into embryos without fertilization and polar nuclei produced endosperm by pseudogamy.     

地塞米松对HepG2细胞分泌载脂蛋白的影响

以培养的人肝癌细胞系HepG2为研究对象,采用“冻干浓缩培养液载脂蛋白测定法”,考察了地塞米松对HepG2细胞载脂蛋白(apolipoprotein,apo)AⅠ、AⅡ、CⅢ、B100及E分泌的影响.结果表明：地塞米松对HepG2细胞apoAⅠ和apoE的分泌有促进作用,对apoAⅡ、apoB100和apoCⅢ的分泌有抑制作用,且这种作用随地塞米松浓度的增加而增强.当培养液中地塞米松的浓度为5.5×10^－5mol/L时,apoAⅠ和apoE的分泌分别增加36.6%和49.4%（P＜0.01）,apoAⅡ、apoB100和apoCⅢ的分泌分别减少38.9%、31.9%和29.8%（P＜0.01）.     

Characterization of a New Chlorophyll-Protein Complex and Studies on Some Properties of Other Chlorophyll-Containing Bands

1. The chlorophyll-protein complexes of sun plant spinach and shade plants Malaxis monophyllos (L.) Sw. and Chlorophytum comosum (Thunb.) Jacques were resolved by SDS-PAGE at lower temperature (2—4 ℃). Besides 8 chlorophyll-containing bands Ⅰa, Ⅰb, Ⅰc, Ⅱa, Ⅱb, Ⅱc, Ⅲ and Ⅳ mentioned in our previous paper (Chu et al., 1980), three more small chlorophyll-containing bands were also observed. Among these small bands Ⅱa which often appeared between Ⅰc and Ⅱa looked like a oligomer of LHCP complex according to its properties in colour, absorption spectrum and fluorescence emission etc. 2. When electrophoresis was carried out at lower temperature (2—4 ℃), the quantity of free pigments (Ⅲ) was obviously lower, while the relative quantities of LHCP Ⅱa, Ⅱb and PS Ⅱ’s band (Ⅳ) were apparently higher than those carried out at higher temperature (12—15 ℃). At lower temperature three bands of Ⅰ could be resolved in shade plants M. monophyllos and C. comosum, and at higher temperature there was only one band of Ⅰ (Ⅰc). But at higher temperature three bands of Ⅰ could be resolved in sunflower. 3. The percentage of LHCP complexes of shade plant M. monophyllos in total amount of chlorophyll (57%) was obviously higher than that of sun plant spinach (43%). The percentage of complexes Ⅰ of sun plant spinach in amount of total chlorophyll (27%) was obviously higher than that of shade plant M. monophyllos (14%). The relative quantity among three bands of Ⅰ in different Plants is different. 4. The chl a/b ratio of LHCP bands of shade plants were lower than that of corresponding bands of sun plants. The chl a/b ratio of Ⅱa of M. monophyllos was 1.1, Ⅱc, 1.2; but that of Ⅱa of spinach was 1.4, Ⅱc, 1.66.     

不同类型海桑-秋茄人工林地上生物量及营养元素积累与分布

海桑(6年生)与秋茄(11年生)人工混交林和海桑、秋茄人工纯林共3种类型(类型Ⅰ、Ⅱ、Ⅲ)地上总生物量分别为38.530、20.012和29.405t·hm^-2,其中类型Ⅰ乔木层占41.0%,灌木层占59.0%,类型Ⅱ乔木层占93.3%,灌木层占6.7%,类型Ⅲ灌木层占100%;生物量年均净积累量分别为4.701、3.380和2.673t·hm^-2·a-1.3种类型10种营养元素总积累量差异明显,分别为765.570、343.925、555.886kg·hm^-2,其中类型Ⅰ乔木层占41.8%,灌木层占58.2%,类型Ⅱ乔木层占92.3%,灌木层占7.7%,类型Ⅲ灌木层占100%;生产单位净积累干物质对营养元素吸收量及营养元素归还率因林分类型各异,类型Ⅰ、Ⅱ、Ⅲ每生产1t净积累干物质净吸收10种营养元素的总量分别为39.860、36.834和18.904kg,而营养元素归还率则分别为61.3%、40.4%和72.2%.     

菜心和水稻绿叶中不同等电点的乙醇酸氧化酶

The proteins with glycolate oxidase activity from B.parachinensis Bailey and rice( Oryza sativa )green leaves were prepared respectively.From the second protein peak on DEAE\|Cellulose column,two glycolate oxidases,expressed as B.parachinensis Bailey GO Ⅲ(specific activity natove 13 2 U·mg -1 ·min -1 )and rice GOⅢ(specific activity 8 8 U·mg -1 ·min -1 ),could not migrate anywhere in 4%～20% native\|PAGE under a pH8.3 buffer system.GOⅢ's p I was about pH8.3. The protein containing B.parachinensis Bailey GOⅢ showed 67±2,43±2,and 38±2 kD in SDS PAGE,band 43±2 kD was the subunit of B.parachinensis Bailey GOⅢ.From the two proteins above,another group of glycolate oxidases,expressed as B.parachinensis Beiley GOⅠ(specific activity 5 U·mg -1 ·min -1 )and rice GOⅠ(specific activity 1 2 U·mg -1 ·min -1 ),showed only one 43±2 kD band in SDS\|PAGE,and was purified on the Sepharose\|6B column which migrated towards anode in the same native\|PAGE showing the M r about 420 kD,or 460 kD and 260 kD respectively.GOⅠ's p I was smaller than pH8.3.Antibody against B.parachinensis Bailey GOⅠ was prepared and its efficacy was about 1/1600 in ELISA.By native\|PAGE,Western blot and rocket immunoelectrophoresis,the third group of glycolate oxidases,expressed as B.parachinensis Bailey GOⅡ and rice G0Ⅱ,were confirmed in crude protein of green leaves and migrated towards cathode under the same native\|PAGE,so GOⅡ's p I was higher than pH8.3.The M r of B.parachinensis Bailey GOⅡ was about 669 kD determined by native\|PAGE Western blot.Rice GOⅠ,rice GOⅢ and rice GOⅡ showed different quantitation under different physiological conditions.Rice GOⅡ could be induced by glycolate.     

Steroidal Alkaloids from Sarcococca vagans

Sarcococca vagans Stapf (Buxaceae) was distributed in Southern Yunnan, China. From the plant collected in Xishuangbanna,three new steroidal alkaloids named vaganines A,B and C( Ⅰ–Ⅲ )together with three known compounds were isolated and on the basis of spectral analyses and chemical evidence, the chemical structures of three new compounds were determined as 20α-dimethylamino-4β-acetoxyl-3β-senecioylamino-5α-pregnane (Ⅰ), 20α-dimethylamino-4β hydroxyl- 3-senecioylamino-△2(3)-pregnaene (Ⅱ), acetate of Ⅱ (Ⅲ); respectively.     

舟山眼镜蛇毒抗肿瘤有效组分分离及其抑瘤作用研究初探

目的从舟山眼镜蛇(Naja atraCantor)蛇毒(snake venom,SV)中分离得蛇毒组分,探讨SV及其分离组分的LD50和抑制肿瘤的作用。方法采用凝胶柱层析方法从蛇毒中分离得到了前Ⅰ1、Ⅰ1、Ⅱ1、Ⅱ2、Ⅲ1、Ⅲ2及Ⅳ等7种组分。采用急性毒性实验、MTT法,研究SV及其7种SV分离组分的LD50和抑制肿瘤的作用。结果 SV经Sephadex G-50层析,可分离为前Ⅰ、Ⅰ、Ⅱ、Ⅲ及Ⅳ5个组分,根据峰面积大小排列:ⅢⅡⅠⅣ前Ⅰ。5个组分再经Sephadex G-25柱层析,可获得7个脱盐组分:前Ⅰ1、Ⅰ1、Ⅱ1、Ⅱ2、Ⅲ1、Ⅲ2及Ⅳ。通过急性毒性实验,明确Ⅳ的毒性最大,其次为Ⅲ2及Ⅲ1,三者的LD50值均低于SV;而Ⅰ1、Ⅱ1、Ⅱ2的毒性均小于SV,前Ⅰ1几乎无毒。SV组分Ⅲ2和Ⅳ的抑瘤作用最强,在高浓度(20μg/ml)时对实验中的2种人肿瘤细胞的抑制率均达到60%以上。结论从SV中分离得到了前Ⅰ1、Ⅰ1、Ⅱ1、Ⅱ2、Ⅲ1、Ⅲ2以及Ⅳ7种组分;组分Ⅳ毒性最强,依次为Ⅲ2Ⅲ1SVⅡ2Ⅱ1Ⅰ1前Ⅰ1;SV及其7种分离组分对2种人肿瘤细胞株(SGC-7901、A549)的生长抑制有一定的特异性,而不同的SV分离组分对同一肿瘤细胞抑制作用亦有差异。     

嗜线虫致病杆菌HB310菌株杀虫蛋白的纯化及活性鉴定

嗜线虫致病杆菌Xenorhabdus nematophila HB310是从河北省土壤中筛选出的一株昆虫病原线虫体内分离纯化获得的共生菌,该菌的发酵液对多种昆虫有较高的杀虫活性。利用85％饱和度的硫酸铵盐析分别获得胞内蛋白提取物和上清液中胞外蛋白提取物,生测结果表明这两种蛋白提取物中都含有胃毒素和血腔毒素。通过制备型非变性凝胶电泳对蛋白提取物进行分离和纯化,得到了3种有杀虫活性的毒素蛋白（毒素Ⅰ、毒素Ⅱ和毒素Ⅲ）,胞内的毒素蛋白与分泌到胞外上清液中的毒素蛋白是同种蛋白。毒素Ⅰ和毒素Ⅱ对棉铃虫初孵幼虫有明显的胃毒活性,但没有血腔毒性;毒素Ⅲ对大蜡螟幼虫有很强的血腔毒性,LD₅₀为0.18 μg/头。SDS-PAGE图谱显示毒素Ⅰ和毒素Ⅱ是由多个多肽组成的复合蛋白,而毒素Ⅲ只分离出一条多肽。毒素Ⅱ在50℃处理10 min,其杀虫活性没有显著变化;70℃处理10 min对毒素Ⅲ杀虫活性没有显著影响。