应用经典热乙醇法从组分IV沉淀中制备白蛋白

将Ｃｏｈｎ氏６法低温乙醇分离人血浆中的组分ＩＶ（ＦＩＶ）沉淀,溶解于注射用水中,加入９５％乙醇后使乙醇浓度为９％,经加温、过滤及超滤制得白蛋白。每公斤ＦＩＶ沉淀可制得白蛋白５７．８ｇ。     

血浆蛋白分离纯化的进展——亲和技术的重要作用

从血浆中分离纯化各种药用蛋白质仍然是生物技术的重要产业。分离纯化技术的进展使得一血多用成为可能 ,大大降低了产品成本。其中 ,亲和技术扮演了重要的角色。经过 2 0多年的进展 ,亲和层析已经从实验室走进产业化 ,以其高选择性、高活性回收率和高纯度等特点 ,成为纯化蛋白质等生物大分子最有效的技术之一。在血浆分离中 ,以乙醇沉淀或离子交换层析预处理后血浆组分为原料 ,用亲和层析可高效地获得目标血浆蛋白。综述了近年来各种亲和层析在血浆蛋白分离制备中的应用 ,并展望了血浆蛋白分离纯化发展的趋势。     

黄附子中糖复合物的初步分析

生药中糖复合物研究是２１世纪生物科学热点之一。本文首次报道了附子中糖复合物的研究结果。我们采用饱和硫酸铵沉淀、乙醇分级沉淀及ＤＥＡＢ－Ｃ３２层析方法,从黄附子中分离出三种组分,通过鉴定发现：组分Ｉ主要为糖蛋白,组分Ⅱ主要含酸性多糖,组分Ⅲ可能是淀粉。此研究结果为全面深入地研究和开发附子提供了参考依据。     

疏水层析结合冷乙醇沉淀纯化人血清白蛋白

将层析技术与冷乙醇工艺相结合用于人血清白蛋白的纯化 ,对各过程所采用的层析介质及层析条件进行了探索 ,得到了一条从人血浆中制备血清白蛋白的新路线 :将一步冷乙醇沉淀后的血浆上清进行脱盐除乙醇 ,用阳离子交换介质CMSepharoseFF以透过式层析的模式吸附非白蛋白组分 ,最后选用ButylSepharoseFF一步疏水层析后所得样品经SDS-PAGE银染显示一条单带 ,分析其纯度大于 99% ,计算工艺收率为 81.2%。与传统冷乙醇工艺相比较 ,该工艺最终样品纯度更高 ,且层析可以在常温下操作 ,易实现自动化控制.     

蝶蛹金小蜂毒液蛋白不同提取分离方法的比较

为了建立蝶蛹金小蜂Pteromalus puparum毒液抑制寄主血细胞免疫活性组分合适的分离纯化方法,就等电点沉淀法、乙醇沉淀法、75%硫酸铵沉淀法、75%硫酸铵沉淀法+40℃加热处理法,以及75%硫酸铵沉淀法分别与3种不同滤膜的分子大小截留法的组合等7种方法对毒液蛋白分离效果及活性的影响进行了比较。结果表明：等电点沉淀法获得的组分抑制寄主菜粉蝶Pieris rapae离体血细胞延展和包囊的活性最强,乙醇沉淀法次之,75%硫酸铵沉淀法最弱。从蛋白组分的SDS-PAGE图谱来看,等电点沉淀法获得毒液组分相对最纯,仅有3条主要谱带,分子量大小在45～116.2 kDa范围内;乙醇沉淀法次之,有5条主要谱带,分子量大小在24～116.2 kDa范围内;硫酸铵沉淀法的谱带组成与毒液蛋白粗提液相似。3种分子大小截留法获得的毒液组分的活性分析表明,强活性组分分子量大小可能都大于100 kDa。综合认为,7种方法中以等电点沉淀法提取分离蝶蛹金小蜂毒液蛋白相对为最适。     

中药桑寄生(Lorathlorace)抗肿瘤毒蛋白的分离及部分性质初步研究

用Sephadex G100分子筛法分离中药桑寄生中蛋白质,得到大分子量组分a和小分子量组分b;用CM-Sepharose Fast Flow分离桑寄生的大分子物质,得到四个部分:组分Ⅰ,Ⅱ,Ⅲ和Ⅳ。对以上各组分蛋白及其分子量用SDS-PAGE电泳确认;选用肝癌细胞Bel-7402,经MTT染色法检测了其抗肿瘤活性。初步得出实验结果:在我国中药桑寄生中分离到的组分Ⅱ(包含两种蛋白或亚基),分子量在31000和33000左右,具有抑制肝肿瘤细胞Bel-7402生长作用;组分Ⅲ中分子量在21000左右的蛋白抗肝肿瘤细胞Bel-7402作用不明显;组分Ⅳ中分子量小于14000的蛋白没有抗肿瘤作用,分子量为36000的蛋白的抗肿瘤作用有待进一步试验确定。     

酵母源葡萄糖耐量因子的提取纯化研究

为探究葡萄糖耐量因子(GTF)分离纯化工艺,简化纯化步骤,以期得到GTF纯品,本实验在前人氨水提取基础上,采用有机溶剂沉淀除去杂蛋白,在有机溶剂的种类、溶剂的浓度、提取组分以及沉淀时间的确定等方面进行了试验,以有机铬含量(μg)与总蛋白含量(mg)的比值为纯化评价标准,高相液相色谱对纯化结果进行验证,同时将纯化前后的GTF作用于胰岛素抵抗型Hep-G2肝癌细胞,测定细胞葡萄糖消耗量,检测GTF纯化品对细胞葡萄糖代谢的调节活性。最终确定用30%低温乙醇沉淀20 min,10000×g离心取上清液分离纯化GTF,此方法相较于氨水直接提取,有机铬含量与总蛋白含量的比值提高了6倍多,GTF提取率和纯度都得到了显著提高,且纯化后的GTF对胰岛素抵抗型Hep-G2细胞葡萄糖代谢具有显著调节作用(P0.01)。     

柱层析法纯化人血纤维蛋白原及其药理功能研究

目的:探讨层析法新工艺和原有的低温乙醇工艺制备纤维蛋白原在大鼠跟腱断裂模型中促恢复的效果差异。方法:构建大鼠跟腱部位断裂模型,将其分为空白组(未剪跟腱)、模型组(跟腱断裂未给药)、实验组(自制纤维蛋白原2 mg/mL)与对照组(市售纤维蛋白原2 mg/mL),观察各组大鼠在手术后三周跟腱部位的最大滑动距离、弹性模量和最大抗拉力差异。结果:采用冷沉淀溶解、酸沉除杂、S/D灭活病毒、MacroCap Q柱层析、过滤等流程可从人血浆冷沉淀组分Ⅰ中成功分离纯度为90.9%纤维蛋白原。试验中构建的大鼠跟腱部位断裂模型无感染、且均存活至试验终止。生物力学结果显示,四组大鼠跟腱在最大滑行距离上无明显统计学差异(P0.05);在跟腱部位弹性模量及最大抗压力比较上,实验组及对照组均优于模型组,但与空白组仍有一定差距,且差异均具有统计学意义(P0.05)。结论:采用柱层析法分离人纤维蛋白原,不仅能有效提高分离效率,减少蛋白损失,还可增强纤维蛋白原在断裂跟腱中的促恢复效果。     

木霉β-1,3-葡聚糖酶的分离纯化

目的:对木霉菌株LE02所产β-1,3-葡聚糖酶的分离纯化方法进行研究。方法:粗酶液分别用硫酸铵、乙醇和丙酮进行沉淀,再用DEAE-Sepharose CL-6B离子交换层析进一步分离纯化,并用SDS-PAGE法测其分子量。结果:硫酸铵分段盐析法沉淀酶蛋白的效果优于乙醇和丙酮沉淀;盐析得到的酶蛋白经透析浓缩后,再经DEAE-Sepharose CL-6B层析分离,可得到单一酶蛋白,总酶活回收率达78.71%,比酶活达到689.9U/mg,提高了53.74倍,经SDS-PAGE法测得该β-1,3-葡聚糖酶的分子量为80.137kDa。结论:采用硫酸铵分段盐析和离子交换层析法可获得电泳纯的β-1,3-葡聚糖酶,且酶活回收率高。     

血浆分段法纵览

<正> 引言 简言之,血浆分段法是从已知质量的血浆中,经济地分离具有适宜纯度和最大产量的一定量血浆组分的一门技艺。 人血浆的工业分段法,起源于第二次世界大战期间,当时Cohn和其同事发展并发表了他们著名的冷乙醇分段工艺。Cohn-OnCley6法和9法应用至今40多年,发挥了非常重要的作用。与此同时,在     

Physical and chemical basis of carbon isotope fractionation in plants

Naturally-occurring variations in the abundances of the stable isotopes of carbon and other elements can be used to understand the dynamics of natural processes in chemistry, biochemistry, biology, medicine, ecology and other fields. The use of carbon-13 isotopic abundances as an indicator of photosynthetic function in plants has become common. The purpose of this article is to describe the physical and chemical processes that contribute to the abundances of carbon-13 in plant materials, and to provide a framework for understanding how those processes control the isotopic contents of natural materials.     

Protein separation by differential drainage from foam

Commercially available beer, which is a dilute solution containing components of yeast, malt, and hop used in the manufacture of the beer, was used as a model system to demonstrate the potential of foam fractionation beyond the primary foaming stage. Most of the components present in the beer concentrated in the initial foam, but they drained differentially in the subsequent collapsed foam collected over a period of 30 min. This resulted in further enrichment, in particular, of components which were present in low concentration in the original beer, Preferential drainage from foam, hence, might provide a novel way of fractionating further the proteins concentrated initially in the liquid films of foam. (c) 1994 John Wiley & Sons, Inc.     

A comparison of fractionation methods for forms of phosphorus in soils

We used l6 soils to compare the Hedley method for soil phosphorus fractionation to an alternative method recently developed by Ruttenberg to differentiate among P fractions in marine sediments. For forms of labile and Fe-bound P in soils, these methods were poorly correlated, with the Hedley fractionation showing a greater ability to discriminate among variations in plant-available P. For Ca-bound P, total organic P, and total P, the methods were well correlated (r² = 0.93, 0.48, 0.74, respectively), although the sum of P measured in the Ruttenberg extractions is only 45% of the total P recovered by the Hedley fractionation. The Hedley fractionation seems superior when an index of plant-available phosphorus and a separation of organic and inorganic forms is needed, whereas the Ruttenberg method allows a separation of CaCO₃-bound P from apatite-P, which is potentially useful in calcareous soils.     

Micropreparation of hemopoietic stem cells from the mouse bone marrow suspension by gravitational field-flow fractionation

Gravitational field-flow fractionation is a relatively simple experimental technique. This method was used for the characterization of stem cells from mouse bone marrow. Because these cells are bigger than the other cells in bone marrow, it is possible to separate them from the mixture. The fractions collected after passing through the separation channel were characterized using a Coulter Counter and used for transplantation into irradiated mice.     

蛋白质沉淀剂对棉铃虫谷胱甘肽S-转移酶的部分纯化

通过用聚乙烯亚胺（PEI）、硫酸铵、聚乙二醇（PEG）沉淀技术和GSH-Sepharose 4B亲和柱对棉铃虫Helicoverpa armigera (Hübner)幼虫中谷胱甘肽S-转移酶进行了部分纯化研究。结果表明PEG10000和PEG20000的纯化效果优于硫酸铵的沉淀效果。通过PEI沉淀去核酸后,再用硫酸铵沉淀,中肠和脂肪体GST活性分布在70%～75％和60%～65％沉淀段,比活力分别为1 081.49和596.41 nmol/(min·mg),纯化倍数分别为2.53和2.2。在6种PEG中,PEG10000和PEG20000的纯化效果较好。在中肠和脂肪体中PEG10000沉淀的GST活性峰分别在40%～45％和30%～40％,GST比活力分别为795.11和1 080.18 nmol/(min·mg),纯化倍数分别是2.4和3.97。PEG20000沉淀中肠和脂肪体GST的活性峰分别在25%～40％和25%～45％,比活力分别是767.57和945.96 nmol/(min·mg),纯化倍数分别是2.81和3.05。用GSH-Sepharose 4B纯化中肠GST,GST比活力达到5 888.44 nmol/(min·mg),纯化倍数达到107.38。     

Effect of pH on successive foam and sonic droplet fractionation of a bromelain-invertase mixture

A droplet fractionation method was previously developed to concentrate a dilute nonfoaming protein solution. In that earlier study with invertase, it was demonstrated that droplets created by ultrasonic energy waves could be enriched up to 8 times that of the initial dilute invertase solution. In this study, a mixture of bromelain (a foaming protein) and invertase (a nonfoaming protein) is investigated as a preliminary step to determine if droplet fractionation can also be used to separate a non-foaming protein from foaming proteins. The foaming mixture containing bromelain is first removed by bubbling the binary mixture with air. After the foam is removed, the protein rich air-water interfacial layer is skimmed off (prior to droplet fractionation) so as not to interfere with the subsequent droplet production from the remaining bulk liquid, rich in non-foaming protein. Finally, sonic energy waves are then applied to this residual bulk liquid to recover droplets containing the non-foaming protein, presumed to be invertase. The primary control variable used in this droplet fractionation process is the pH, which ranged for separate experiments between 2 and 9. It was observed that the maximum overall protein partition coefficients of 5 and 4 were achieved at pH 2 and 4, respectively, for the initial foaming experiment followed by the post foaming droplet fractionation experiment.     

Proteases from the fungus Metarhizium anisopliae toxic for Galleria mellonella larvae

The high molecular fraction of the extract from Metarhizium anisopliae grown on wheat bran contains proteolytic enzymes which are toxic for Galleria mellonella larvae. The complex of proteases was fractionated using precipitation with ammonium sulfate, gel filtration, and electrofocusing. Two components have been found: one with the optimum of activity on hemoglobin at pH 6.5, and the second with the optimum around pH 9. The prevailing protease acting at pH 6.5 was inhibited by phenylmethylsulfonyl fluoride and the inhibition was followed by decrease of toxicity. The molecular weights of the enzymes are 35 × 10³ and 71 × 10³.     

Localization of [14C]DDT in the ventral nerve cord of the cockroach,Periplaneta americana (L.)

[¹⁴C]DDT was used as a probe to determine the subcellular localization of DDT in the ventral nerve cord (VNC) of the cockroach, Periplaneta americana (L.). Male cockroaches were injected intra-abdominally with [¹⁴C]DDT and their VNCs removed at 1 h post-injection. The VNCs were then subjected to homogenization and differential centrifugation to isolate plasma membrane, mitochondrial, and microsomal fractions. Results indicate that the plasma membrane fraction contained the greatest amount of [¹⁴C]DDT, with the mitochondrial and microsomal fractions containing significantly less. Calculations and a comparison with I₅₀ values for oligomycin-sensitive (OS)Mg-ATPase from the literature support the prediction that an insufficient amount of DDT reaches the ventral nerve cord mitochondria of a cockroach to effect an I₅₀ level of inhibition of the (OS)Mg-ATPase.     

Separation of human and animal cells by steric field-flow fractionation

In this work, the feasibility of separating and characterizing cell populations by steric field-flow fractionation (steric FFF) is demonstrated by application to fixed human and avian red cells, fresh blood from several species, and viable HeLa cells. The basis for this work is established by means of a discussion of the role of steric FFF in the broad family of field-flow fractionation techniques. The behavior of steric FFF is then characterized by application to standard polystyrene latex beads and to fixed red blood cells. Studies of these standards and of the other cells noted under various conditions of field strength and flow velocity are used to improve the separation conditions and approach optimization. It is shown that the fixed human and avian red cells can be separated in a time of less than 15 min. In addition, it is shown that HeLa cells maintain their viability after passage through the separation channel.     

Characterization of Lead in Soils of a Rifle/Pistol Shooting Range in Central Florida,USA

The distribution of lead in soil samples collected from both surface (0 to 10?cm) and profile (O 0 to 10?cm, E 11 to 30?cm, Eb 31 to 50?cm, Bw 51 to 100?cm, and C 181 to 200?cm) at a 14-year-old rifle/pistol shooting range located in central Florida were determined using EPA Method 3051a (microwave, HNO₃/HCl=3:1, v/v). In addition to total lead analysis, Toxicity Characteristic Leaching Procedure (TCLP) analysis was performed on corresponding samples to determine whether the soils would require special handling as hazardous waste if the soils were to be removed from the range. Total lead in surface soils varied from 330 to 17 850?mg Pb kg^?1, with the greatest concentration in the middle of the backstop berm. The TCLP tests indicated that lead in all surface soils exceeded the 5?mg Pb L^?1 critical level of federal regulation for solid wastes and hazardous wastes provided by the Resource Conservation and Recovery Act (RCRA) and would be characterized as hazardous waste. Sequential fractionation and X-ray diffraction (XRD) analyses revealed that lead carbonate existed predominantly (91.3%) in the berm soil. The weathering of lead bullets in the soil environments formed primarily as hydrocerussite (Pb₃(CO₃)₂(OH)₂), with small amounts of massicot (PbO) and cerussite (PbCO₃). However, the elevated soil pH, caused by the oxidization and transformation process of elemental lead in lead bullets, could be a significant factor in limiting the migration of lead in the soil.