聚乙二醇诱导鸡红细胞融合条件的优化

目的:探讨聚乙二醇诱导鸡红细胞融合最适条件.方法:以鸡红细胞为材料,聚乙二醇为诱导剂,从细胞密度、融合温度、聚乙二醇浓度及反应时间进行单因素实验,并设计3因素3水平的正交实验计算细胞融合率.结果:鸡红细胞融合的最佳条件是:细胞密度为2×106个/ml,聚乙二醇浓度为35%,反应温度为35℃,反应时间40min.结论:在该条件下,细胞融合率最高达33.06%.     

鸡红细胞融合最适条件的探讨

目的：探讨快速、有效的细胞融合条件.方法：用鸡红细胞为材料,聚乙二醇（Mw=4000）为诱导剂,诱导鸡红细胞融合.结果：鸡红细胞融合的最适温度为39℃,最适时间为15min.结论：在该条件下,同时用Giemsa染液对融合细胞染色,实验观察效果明显.     

鸡红细胞融合最适条件的探讨

目的:探讨快速、有效的细胞融合条件。方法:用鸡红细胞为材料,聚乙二醇(Mw=4000)为诱导剂,诱导鸡红细胞融合。结果:鸡红细胞融合的最适温度为39℃,最适时间为15min。结论:在该条件下,同时用Giemsa染液对融合细胞染色,实验观察效果明显。     

聚乙二醇丙烯酸酯的合成与表征

以聚乙二醇-400（PEG400）与丙烯酸直接缩合反应,在不加有毒带水剂的条件下合成了丙烯酸聚乙二醇酯（PEGA）。通过正交实验确定酯化反应的最佳条件：丙烯酸／PEG400的摩尔比为2．0：1．0,反应温度是110℃,阻聚剂对苯二酚为0．4％（以醇酸总质量计）,反应时间为6小时,催化剂对甲苯磺酸为0．8％（以醇酸总质量计）,产率为76．7％。产品结构经IR和1HNMR表征,证明是所需的产物。     

海滨锦葵油制备生物柴油工艺条件优化

以海滨锦葵油为原料制备生物柴油。通过单因素试验及正交试验研究了反应温度、催化剂用量、醇油摩尔比、反应时间、搅拌强度等因素对酯交换率的影响。结果表明,在试验范围内各影响因素对酯交换率作用的大小依次为：搅拌强度＞催化剂用量＞醇油摩尔比＞反应时间＞反应温度。海滨锦葵油制备生物柴油的最佳工艺参数为：搅拌强度为1800r.min-1,催化剂KOH用量为海滨锦葵油质量的1%,醇油摩尔比6/1,反应时间60min,反应温度65℃,在该工艺条件下,酯交换反应三次,酯交换率达到97.8%。     

聚乙二醇修饰重组人生长激素的初步研究

目的 探讨聚乙二醇(MW20kD)修饰重组人生长激素(rhGH)的反应条件以及修饰产物的纯化方法。方法在不同条件下,将聚乙二醇活性酯与rhGH反应,以单个PEG-GH的比例为指标,用SDS-PACE和薄层扫描方法,确定其在反应产物中所占的比例;采用CM-Sepharose FF离子交换和Sephacry 1S-200分子筛凝胶层析法对修饰产物进行分离纯化。结果聚乙二醇修饰rhGH的反应条件为pH8．0、rhGH与聚乙二醇的比例1：2(mg：mg)、反应时间2．0h;反应产物经两步纯化,所得的单个PEG-GH纯度大于95％。结论 初步确定了聚乙二醇修饰rhGH的反应条件和修饰产物的纯化方法。     

氢氧化钠法提取虾壳蛋白最佳条件的研究

利用蛋白质的盐析原理对虾壳蛋白进行分离.先分别以氢氧化钠的浓度、反应时间、反应温度作为变量进行单因素分析,并据此结果进行三因素三水平的正交试验分析,确定出提取龙虾壳蛋白质的最佳实验条件为:反应温度100℃、氢氧化钠浓度10%、反应时间4 h,继而在此条件下检验出所提取的蛋白质的纯度为77.38%.     

双氧水介导制备对硝基苯甲酸乙酯的初步研究（英文）

目的：探讨双氧水催化合成对硝基苯甲酸乙酯的可行性,并考察了反应物的摩尔比、催化剂用量、反应温度及反应时间对产物收率的影响。方法：分别采用单因素设计实验与正交设计实验,分析比较这两种方法的最佳反应条件。采用数字熔点仪测定样品的熔点;用GC112A型气相色谱仪测定了产物的纯度;用傅里叶变换红外光谱仪测定产物的结构。结果：双氧水可以作为合成对硝基苯甲酸乙酯的催化剂。综合分析可知：当无水乙醇和对硝基苯甲酸的摩尔比为4：1,催化剂含量为10%,反应温度为80℃,反应时间为2.5-3h时酯化产率可达到最高值。结论：双氧水催化对硝基苯甲酸、无水乙醇合成对硝基苯甲酸乙酯的效率较高,产品纯度高,环境污染小,不失为一种新的合成方法。     

Mg^2＋浓度对细胞融合效果的影响

目的：细胞融合是细胞生物学中一种常用的技术,有着广泛的应用,如单克隆抗体制备,核质研究,疫苗研发等。其中,聚乙二醇（PEG）化学融合是最为常用的一种细胞融合技术,影响PEG化学细胞融合效果的因素有很多,但是对一些具体因素的研究的不是很全面。本文旨在为了更全面的了解PEG诱导的化学细胞融合的影响因素,优化融合条件,以此扩大PEG化学融合应用范围。方法：以鸡血血红细胞为材料,通过调节已有的Hanks融合液中镁离子浓度,比较各实验组以及对照组的细胞融合率,探究了Mg^2＋浓度对细胞融合效果的影响,确定了为提高细胞融合效率应使用的Mg^2＋浓度区间。结果：可以在原有的Hanks配方的基础上,调节Mg^2＋浓度至10 mmol/L-20 mmol/L这个范围,细胞融合率较大。结论：Mg^2＋对细胞融合有一定影响,通过调节Mg^2＋浓度至上述合适区间可以达到较高的细胞融合率,从而为PEG化学融合提供了一种优化方案。     

正交设计法研究壳聚糖降解液的制备工艺

选择反应温度、反应时间、双氧水重量百分浓度3个影响因素,采用对真菌的抑制效果为评价指标,对壳聚糖降解液制备工艺进行了研究。试验结果表明,以60℃、4 h、双氧水重量百分浓度10%为最佳工艺条件。     

葡萄糖浓度对细胞融合效果的影响

目的:细胞融合是细胞生物学领域近30年来得到迅速发展的一项新兴技术手段,因其操作简便、人工可控等优点在研究核质互作、肿瘤发生、疫苗研发和培育新型生物品种等方面均有广泛应用。其中,利用聚乙二醇(PEG)进行化学融合是细胞融合中最为常用且简便的技术手段。PEG化学融合效果受到多种因素影响,如PEG浓度、Ca2+、Mg2+、pH值等,然而对于糖类物质在细胞融合中的影响未见报道。本文旨在为了更全面了解PEG法诱导的化学细胞融合,通过优化融合条件以提高化学细胞融合效率。方法:选取鸡血血细胞为材料,通过改变原Hanks缓冲液中葡萄糖浓度,观察比较各组细胞融合率,探究葡萄糖浓度在化学细胞融合中的影响,并通过对比结果获得了对于鸡血血细胞应采用的最适葡萄糖浓度区间。结果:对于鸡血血细胞融合实验,葡萄糖浓度在10-14 mmol/L范围内细胞融合效率较原Hanks液配方高2倍左右。结论:葡萄糖对细胞融合效果具有一定的影响,可以通过调节葡萄糖浓度提高细胞融合率,从而为PEG化学细胞融合提供一种更为优化的方案。     

狂犬疫苗单克隆抗体制备过程中细胞融合条件的探索

在充分了解SP2/0细胞系的生长、增殖和遗传特性后,以聚乙二醇(PEG)诱导动物细胞融合为契机,意在探索不同分子量、不同浓度的PEG作融合剂对诱导SP2/0细胞与脾细胞融合的最适条件,在HAT选择培养基下通过细胞融合率的变化进行比较。结果表明,分子量为4000,浓度为50%的PEG诱导的细胞融合率最高,为下一步制备狂犬病毒疫苗单克隆抗体奠定基础。     

Single-Pair Fusion of Various Combinations Between Female Gametoplasts and Other Protoplasts in Nicotiana tabacum

This paper reports an enzymatic maceration-osmotic shock method for isolation of tobacco embryo sac and its component cell protoplasts, and also a new method for fusion between single pairs of selected mesophyll protoplasts using polyethylene glycol (PEG) as on inducing agent. An integration of these two methods has led to the successful fusion of female gametoplasts with other kinds of protoplasts. The female gametoplasts described here, in a broad sense, include the egg cell (E), central cell (C) and synergid (S). One of the female gametoplasts was selected and fused with another female, male (generative cell, G) or somatic (mesophyll, M)protoplast. Various combinations were involved: E+S, E+C, E +G, E+M, C+C, C+S, C+G, C+M, S+S, S+G, S+M, etc. Briefly, the authors were able to choose any desired combination to realize single-pair fusion by the new PEG method. For the purpose of culturing such fusion products that were limited in number, the authors had done some preliminary experimets using mesophyll protoplasts as feeder cells. Two methods were adopted: the microdrop culture, and the millicell culture with feeder cells. The mesophyll protoplasts were precultured for 2—3 days in large for population expansion before they were used as feeder cells. One or several protoplasts were cultured in a microdrop or a millicell and were induced formation of small cell clusters. This result indicated that the culture methods might also be suitable for culturing the products from fusion of female gametoplasts and other protoplasts in this plant species.     

Trout red blood cells treated with proteases fuse when placed on glass slides

Treatment of trout red blood cells (RBC) with proteases and polyethylene glycol (PEG) either successively or concurrently caused cell fusion. Neither PEG nor protease treatment alone brought about the fusion of cells in suspension. However, incubation of RBC on glass slides with proteases caused extensive fusion.     

Phytohemagglutinin-enhanced hybrid colony formation by cells from aged mice: Expression of th 4mod-1 mouse locus in human-mouse hybrids

Summary Cells from a continuous human line and freshly isolated cells from old adult mice heterozygous at theMod-1 locus were fused in the presence of polyethylene glycol (PEG). The production of hybrid cells, as a function of PEG concentration in the presence and absence of phytohemagglutining (PHA), was measured by cell survival and proliferation on selective medium. The incorporation of PHA into the fusion mixture allowed cell fusion to take place at nontoxic concentrations of PEG. PHA increased the frequency of cell fusion and increased the production of viable hybrid cells from 138- to over 2800-fold depending on cell type. The results suggest that the procedure may have broad application in promoting the fusion of cells sensitive to PEG. Clones were analyzed for isozymes of malic enzyme and glucose-6-phosphate dehydrogenase. The expression of the gene encoding X-linked mouse glucose-6-phosphate dehydrogenase confirmed that the cells were hybrids. These cells lost other mouse isozymes rapidly. In those clones in which the mouse malic enzyme gene was expressed, the product ofMod-1 ^α was detected significantly more frequently than that ofMod-1 ^b.     

Effects of pH on cell fusion induced by electric fields

Electrofusion has recently become an important area of cell biology research. We studied the effects of pH of the cell medium on the electrofusion of human red blood cells. Cell fusion was monitored by observing the movement of a lipophylic dye between neighboring fused cells using a fluorescence microscope. The cells were first brought into close contact by dielectrophoresis. Fusion was then induced by three pulses of high-intensity electric field. Within minutes following the pulse application, many cells were observed to fuse together to form fusion chains of different lengths. We found that the optimal pH for cell fusion is around pH 7.5. At this pH, the fusion yield was highest (ranging from 57 to 81%) and the average number of cells within a fusion chain was also the largest. The dependence of cell fusion on pH is more sensitive at low than at high pH. The fusion yield was decreased by 40% when the pH was changed from 7.5 to 6.0, but there was only a 20% decrease in yield between pH 7.5 and 10.0 We suspect that the observed pH effects may be caused by a redistribution of fixed charges at the cell surface, or changes in amphipathicity of the surface proteins.     

A simple assay for optimizing yeast-mammalian cell fusion conditions

Polyethylene glycol (PEG)-induced cell fusion can be a useful method for the transfer of yeast artificial chromosomes (YACs) from yeast spheroplasts to mammalian cells in culture, although success varies between recipient cell types. Experiments aimed at determining optimum fusion conditions can also be very time-consuming. To minimize this difficulty, a reporter plasmid has been constructed that allows yeast-mammalian cell fusion rates to be determined within 3 d. The speed and sensitivity of the assay should allow a more systematic evaluation of cell lines for their capacity to fuse with yeast, and for rapid optimization of fusion parameters.     

转人生长激素鼠胚成纤维细胞的暂态表达方法的初步确立

探讨作为转基因克隆动物核供体的、不具备分泌人生长激素（hGH）功能的转hGH鼠胚胎成纤维细胞（tEF）体外表达人生长激素的简便的暂态表达方法。首先,转染,3d后筛选出G418,与无hGH分泌的人乳腺癌细胞株（MCF-7）在聚乙二醇（PEG）作用下融合,培养1～2d,放射免疫分析方法检测相同数量的MCF-7组、转染MCF-7组、tEF组以及融合细胞共4组培养液中hGH的表达。结果显示tEF组和MCF-7组均无hGH表达;二者的融合细胞组培养液中hGH表达量可高达0.84mIU/L。可见,不表达hGH的tEF与MCF-7融合形成的杂种细胞,可作为暂态表达系统检测转基因细胞的表达。