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目的优化桦褐孔菌提取工艺,提高桦褐孔菌多糖得率。方法首先对桦褐孔菌多糖提取的主要影响因素纤维素酶用量、酶解温度、溶剂倍量、酶解时间、pH值进行单因素条件筛选。然后采用正交设计法对影响纤维素酶辅助提取多糖的条件进行优化。结果最佳提取条件为:料液比1:40、酶解时间60 min、酶解温度50℃、加酶量0.15 g、酶解pH=5.0。结论纤维素酶对桦褐孔菌多糖进行辅助提取,相比传统的热水浸提,能够显著提高桦褐孔菌多糖的提取率,比水浸提高29.07%,是一种较为有效的提高多糖得率的方法。 相似文献
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目的:优选杜仲叶绿原酸的提取工艺。方法:采用单因素试验考察酶解pH、酶解时间、酶解温度、酶用量、固液比、超声时间、超声提取温度对绿原酸提取率的影响。以绿原酸提取率为指标,以超声提取时间、固液比、酶解温度和酶用量为考察因素,采用正交试验优选杜仲叶绿原酸的提取工艺。结果:优选工艺为提取时间40 min,固液比1∶15(g/ml),酶解温度45℃,酶用量20mg,绿原酸提取率为2.37%。结论:优选的工艺合理、可行,具有提取率高、节能等优点,可为工业化生产提供参考。 相似文献
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目的 研究从枇杷果渣中提取果胶的最佳条件.方法 以不同的酸进行酸解,再进行正交试验以优化提取条件.结果 亚硫酸(H2SO3)是最适宜的酸解剂.结论 从枇杷果渣中提取果胶的最佳条件为:pH1.5、提取温度95℃、提取时间2.0h、固液比1∶30,在该条件下,果胶得率为15.29%,经脱色、脱蛋白、透析、盐沉淀、脱盐、洗涤干燥后,果胶得率为9.50%. 相似文献
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目的:以单因素实验和响应面法优选葛根总蛋白的提取工艺.方法:采用Tris-HCl溶液提取葛根总蛋白;Folin-酚法测定提取液中的蛋白质含量;凯氏定氮法测定葛根粉中蛋白质含量及提取率.以葛根蛋白提取率为指标,以提取液的pH、提取温度、液料比、Tris-HCl浓度、提取时间为因素,通过单因素实验确定因素水平,利用响应面法,通过三因素(提取液pH、提取温度、液料比)三水平实验设计,对葛根蛋白的提取条件进行优化,最终优化出葛根药材蛋白质的最佳提取条件.结果:葛根蛋白提取的最优条件为:提取时间60 min,Tris-HCl浓度为50 mmol·L-1,pH 8.6,料液温度为48℃,液料比为22:1(mL·g-1),蛋白提取率为35.33%.结论:该优化工艺收率高,具有较好的稳定性和工艺可行性. 相似文献
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目的 优化酶解-吸附澄清法提取水辣蓼总黄酮的工艺.方法 采用响应面法,构建多元二次回归数学模型,筛选酶法提取和絮凝澄清的最佳工艺条件.结果 最佳酶法提取工艺为料液比1∶50,pH6.06,复合酶用量0.24%,酶解温度50℃,酶解时间1.62 h;最佳澄清工艺为酶解液的浓缩比1∶5,药液pH5.24,膨润土用量0.45 mL·g-1,43.43℃下絮凝40 min.结论 酶法提取条件温和,膨润土絮凝能有效降低酶解液中总固形物的含量,优于传统醇沉法. 相似文献
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超声波复合酶法提取软紫草多糖的工艺优化 总被引:1,自引:0,他引:1
目的研究超声波复合酶法提取软紫草多糖的最佳工艺条件。方法采用单因素分析和正交试验,以软紫草提取物中多糖得率和多糖含量为综合评价指标,考察超声波复合酶法中主要因素对软紫草多糖提取效果的影响。结果超声波提取优化工艺条件为:超声处理时间40 min,料液比1∶12,功率160 W;在超声波优化结果基础上,进一步进行超声波复合酶法处理,酶解最佳提取条件为酶解时间40 min,酶解温度55℃,pH 5.5,纤维素酶、果胶酶、蛋白酶添加量均为2%。结论超声波复合酶法双重处理可显著提高软紫草多糖的提取效果。 相似文献
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目的 采用超声波辅助提取苗药用的土人参根中总黄酮,比较不同提法所得总黄酮的抗氧化活性。方法 在单因素试验基础上采用响应面法优化超声波处理后固液比、乙醇体积分数、浸提温度及其交互作用对总黄酮得率的影响,DPPH.、超氧阴离子与羟基自由基清除法考查水浴、超声波辅助和酶辅助提取的苗药土人参根中总黄酮的抗氧化活性。结果 苗药用土人参根中总黄酮的最佳工艺为固液比1:26、乙醇体积分数65%、浸提温度70℃,在此条件下,总黄酮得率为 2.62% ,与回归方程预测值 2.603% 符合良好。结论 该优化工艺实现了土人参根中黄酮类化合物的高效提取,所得总黄酮以酶法提取的抗氧化性能力最强。目的 采用超声波辅助提取苗药用的土人参根中总黄酮,比较不同提取方法所得总黄酮的抗氧化活性。方法 在单因素试验基础上采用响应面法优化超声波处理后固液比、乙醇体积分数、浸提温度及其交互作用对总黄酮得率的影响,DPPH?、超氧阴离子与羟基自由基清除法考查水浴、超声波辅助和酶辅助提取的苗药土人参根中总黄酮的抗氧化活性。结果 苗药用土人参根中总黄酮的最佳工艺为固液比1:26、乙醇体积分数65%、浸提温度70℃,在此条件下,总黄酮得率为 2.620% ,与回归方程预测值 2.603% 符合良好。三种提取方法所得总黄酮的抗氧化活性以酶法提取的最强且均好于Vc。结论 该优化工艺实现了土人参根中黄酮类化合物的高效提取,不同提取方法得到的总黄酮抗氧化活性差异明显。 相似文献
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历代本草有关九香虫的记载较多,但描述较为简略,且部分混淆品与其形态相似,导致目前九香虫商品品种混乱,需要深入开展九香虫的本草考证.目前九香虫野生资源骤降,人工养殖规模尚未形成,亟待寻找新药源.本文通过查阅历代中医药典籍、炮制规范,结合现代研究,对九香虫的名称、基原、性味归经、主治功效、炮制沿革进行系统的考证,对九香虫混... 相似文献
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T C Lee P L Chello T C Chou M A Templeton J C Parham 《Journal of medicinal chemistry》1983,26(2):283-286
An N-aminated pyrazine analogue of cytidine, in which the pyrimidine N(3) ring nitrogen and C(4) amino group were replaced by a C-amino and an N-amino function, respectively, was prepared as a potential deaminase-resistant cytidine antimetabolite. The nucleoside 1,2-diamino-4-beta-D-ribofuranosylpyrazin-2-onium chloride (6) was a mild cytostatic agent but was neither a substrate for nor an inhibitor of mouse kidney cytidine deaminase. It ionized with a lower pKa than expected. The anion did not undergo the dimerization usually observed with N-imino heterocyclic ylides but unerwent hydrolysis of the 2-amino group to yield a 1-aminopyrazine-2,3-dione nucleoside. 相似文献
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中国毛虾ACE抑制产物的酶法制备及其降低原发性高血压大鼠血压的效果(英文) 总被引:2,自引:1,他引:2
目的利用中国毛虾制备具有ACE抑制活性及抗高血压活性的酶解产物。方法采用体外试验法检测中国毛虾5种常用蛋白酶酶解产物的ACE抑制活性,筛选出一种蛋白酶作为酶法制备中国毛虾ACE抑制产物用酶,并对其作用条件进行正交优化,利用原发性高血压大鼠评估酶解产物的抗高血压效应。结果胃蛋白酶优化后的酶解条件是:pH 2.4,温度41℃,酶解时间3 h,酶/底物比(E/S)3%,底物浓度8%。以该条件制备的酶解产物对ACE的抑制活性为IC500.65 mg/ml,以1.0 g/kg体重的剂量喂食原发性高血压大鼠4 h后收缩压降低3 886 Pa(29mmHg)。结论中国毛虾的胃蛋白酶酶解产物具有较强的ACE抑制活性及抗高血压活性。 相似文献
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山羊角提取物中氨基酸的种类研究与含量测定 总被引:1,自引:0,他引:1
目的研究山羊角提取物中氨基酸的种类和含量,为建立山羊角提取物质量控制提供依据。方法采用分子排阻色谱法检测山羊角提取物中物质的分子量范围。利用稳定同位素iTRAQ标记/液质联用法对山羊角提取物进行42种全谱氨基酸检测。结果山羊角提取物中物质的分子量范围在50389 Da。090903批、090904批、091001批山羊角提取物中分别包含34种氨基酸(蛋白质氨基酸19种、非蛋白氨基酸15种),31种氨基酸(蛋白质氨基酸19种、非蛋白氨基酸12种)、33种氨基酸(蛋白质氨基酸19种、非蛋白氨基酸14种),山羊角提取物中未检出多肽及大分子物质。天门冬氨酸及谷氨酸加热易破坏,故在提取物制备过程中应严格控制干燥时间和温度。结论本研究建立了快速、稳定检测山羊角提取物中42种全谱氨基酸种类及含量的方法,为建立山羊角提取物质量检测标准提供参考依据。 相似文献
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目的探讨胃蛋白酶水解黄粉虫蛋白制取复合氨基酸液的工艺。方法以黄粉虫为原料,以碱法提取黄粉虫蛋白,采用胃蛋白酶水解黄粉虫蛋白制取复合氨基酸液。通过单因素试验探讨了底物浓度、pH值、酶浓度、水解温度及水解时间与水解率的关系,采用正交试验L16(4^5)优选水解工艺条件。结果最佳酶解工艺条件为:底物浓度为1∶5,pH值4.0,酶浓度1.5%,水解温度60℃,水解时间5 h。水解率达到24.15%。结论按最佳条件水解完毕后,通过酶灭活,中和,脱色等处理可得到黄色澄清的黄粉虫蛋白复合氨基酸液。所制得的复合氨基酸种类齐全,必需氨基酸含量高。 相似文献
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N-Hydroxysulfosuccinimide esters are reactive functional groups employed in a variety of protein modification reagents, especially cross-linking reagents. For these compounds, hydrolysis is the most important reaction competing for reaction of the esters with nucleophilic groups in proteins. We have employed model compounds to investigate the rates of hydrolysis of N-hydroxysulfosuccinimide esters and their reactions with the α-amino group and the side chains of naturally occurring amino acids, under conditions comparable to those used for protein modification studies. The rates of hydrolysis observed were found to be very low, as compared with their rates of reaction with nitrogen nucleophiles found in proteins. Further, within the ranges investigated, the rate of aminolysis was observed to increase more rapidly than the rate of hydrolysis with increasing pH or with increasing temperature. Four amino acid side chains and the α-amino group were found to react measurably with N-hydroxysulfosuccinimide esters. At pH 7.4 and room temperature, the order of reactivity was found to be Nα-Cbz-histidine < Nα-Cbz-lysine ≤ phenylalanine (α-amino group) ?N-acetylcysteine ?N-acetyltyrosine; however, the acylimidazole adduct formed with the side chain of histidine was found to be a transient product, subject to hydrolysis or reaction with another nucleophile. 相似文献
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Selective inhibition of excitatory amino acid-stimulated phosphoinositide hydrolysis in the rat hippocampus by activation of protein kinase C 总被引:4,自引:0,他引:4
The relative roles of protein kinase C in regulating excitatory amino acid-, cholinoceptor-, and adrenoceptor-stimulated phosphoinositide hydrolysis were studied. Slices of rat hippocampus were prelabeled with [3H]-myo-inositol, and agonist-induced [3H]-phosphoinositide hydrolysis was measured by the formation of [3H]-inositol monophosphate ([3H]-IP) in the presence of lithium ion. Activation of protein kinase C with phorbol 12,13-dibutyrate (PDB) (10(-6) M) completely inhibited ibotenate (IBO) (10(-3) M)-induced [3H]-phosphoinositide hydrolysis. Half-maximal inhibition was observed at about 10(-7) M PDB. Higher concentrations of PDB were required to inhibit stimulation of [3H]-IP by either carbachol (CARB) (10(-3) M) or norepinephrine (NE) (10(-4) M, and only partial inhibition could be attained. Preincubation with staurosporine (STAURO) (10(-5) M) or 1-(5-isoquinolinesulfonyl)-2-methylpiperazine (H-7) (10(-4) M), inhibitors of protein kinase C, potentiated IBO- but not CARB- or NE-induced stimulation of [3H]-IP. PDB inhibition of IBO- or NE-stimulated [3H]-phosphoinositide hydrolysis was reversed by co-addition of STAURO or H-7. In the case of IBO + STAURO, this reversal was to the potentiated level observed with STAURO alone. Enhanced agonist stimulation and reversal of PDB inhibition were also produced by STAURO when [3H]-phosphoinositide hydrolysis was stimulated by either L-glutamate or quisqualate. These experiments show that direct activation of protein kinase C by PDB leads to inhibition of phosphoinositide hydrolysis mediated by excitatory amino acid receptors, cholinoceptors, or adrenoceptors. However, the enhanced agonist-stimulated phosphoinositide hydrolysis elicited by inhibitors of protein kinase C suggests that, when protein kinase C is indirectly activated, only excitatory amino acids rapidly inhibit further receptor-coupling. 相似文献
