角蛋白水解液中L-胱氨酸含量测定方法的比较研究

比较研究了用碘量法和分光光度法测定角蛋白水解液中Ｌ－胱氨酸含量的适用性。结果表明,磺量法不适用于水解液中Ｌ－胱氨酸含量的测定。分光光度法不仅适用于水解液中Ｌ－胱氨酸含量的测定,同时也适用于产品Ｌ－胱氨酸含量的测定,测定结果准确可靠,相对误差为０．２９％～０．８４％。     

紫外可见分光光度法测定杜仲绿原酸含量的方法研究

目前,测定绿原酸含量的方法很多,常采用毛细管电泳法、ＨＰＬＣ法、可见分光光度法和纸层析-紫外可见分光光度法等[1,2,3,4]。但样品处理均采用索氏回流提取,后经层析分离洗脱等步骤,时间长、效率低。本文采用紫外可见分光光度法测定绿原酸含量,只需超声波提取一小时,不经...     

广西不同产地番石榴叶总黄酮含量测定

目的对广西不同产地番石榴叶中总黄酮含量进行测定。方法应用紫外分光光度法,以芦丁为对照品,于357nm下测定吸光度,计算番石榴叶中总黄酮的含量。结果在1.7~14.3范围内总黄酮含量与吸光度A值线性关系良好,平均回收率=99.28%,RSD=3.69%,R2=0.9993。结论该方法简便可靠、快速、重现性好,适用于番石榴叶总黄酮含量测定。采收地区不同,番石榴叶中总黄酮的含量也不同。     

分光光度法测水红花子中花旗松素含量

目的:检测水红花子中花旗松素的含量.方法:采用紫外分光先度法,在常温下(25℃)290nm处,对水红花子乙醇提取物进行吸光度测定.结果:此方法线性范围:0.002～0.01 g/L,花旗松素浓度与吸光度线性关系:y=0.0724x 0.007,r2=0.9986;平均回收率为99.37%,RSD=0.897%.结论:紫外分光光度法测定水红花子中花旗花素合量操作简便、快速和准确度高,具有一定实用价值.     

牡蒿总黄酮提取方法的研究

采用水浴法、超声波法和索式提取法,分别提取牡蒿总黄酮,以紫外分光光度法在510nm下测定其含量,以提取液中黄酮含量为标准,设置正交试验对提取条件和工艺进行研究.结果表明:以85%甲醇溶液索氏提取2h得率最高;70%乙醇溶液提取6h次之,但最适用于工业和食品生产.     

静脉注射人免疫球蛋白中IgG含量的测定方法的比较

目的:对IgG的检测方法———紫外分光光度法和免疫单扩散方法进行比较。方法:采用紫外分光光度法和免疫单扩散法对样品进行IgG含量测定,然后对结果进行分析。结果:两种方法测定的结果差异无显著性(P>0.05)。紫外分光法操作更方便、快捷,准确。     

分光光度法测定灵芝三萜含量的干扰因素探讨

根据药典方法,以齐墩果酸为对照品,对灵芝中含有的三萜、甾醇和脂肪酸3种类型化合物进行分光光度法测定,并对影响三萜含量测定的因素进行分析。结果表明灵芝中的甾醇和脂肪酸类化合物会干扰所有的测定结果,尤其影响灵芝孢子中三萜含量的测定。灵芝子实体中三萜化合物的结构特征,造成了其测定值远远低于真实值。因此,分光光度法不适用于测定灵芝子实体、菌丝体和孢子及其相关产品中的三萜含量。     

紫外分光光度法测定肉碱转化液中巴豆甜菜碱的含量

通过对巴豆甜菜碱和L－肉碱在紫外188－215mm的光吸收的比较,建立了紫外分光光度法测定肉碱转化液中巴豆甜菜碱含量的方法,测定波长205mm,线性范围0－25ug/ml,该方法快速方便 ,重复性好,可用于L－肉碱生产过程中巴豆甜菜碱的跟踪检测。     

重组人糖基化单链尿型纤溶酶原激活剂中试生产中蛋白含量测定方法的比较

在单链尿型纤溶酶原激活剂中试生产中 ,用不同的方法对产品蛋白含量进行测定 ,得到的结果常常存在很大差异。通过对紫外法和 Lowry法的比较分析 ,我们认为紫外法更适用于单链尿型纤溶酶原激活剂生产中的产品的蛋白含量测定     

旋光法测定盐酸麻黄碱滴鼻液的含量

盐酸麻黄碱为肾上腺受体激动药,有收缩血管的作用,盐酸麻黄碱滴鼻液在临床上广泛应用。它的含量测定方法有中和滴定法、紫外分光光度法。根据盐酸麻黄碱有旋光性的特点,本文试用旋光法测定盐酸麻黄碱滴鼻液的含量,结果满意。     

Inhibiting the color formation by gradient temperature‐elevating Maillard reaction of soybean peptide‐xylose system based on interaction of l‐cysteine and Amadori compounds

Light color and savory flavor enhancer are attractive for consumers and food producers. The effect of addition time of l ‐cysteine on inhibiting color formation was investigated in soybean peptide‐xylose system, and the possible pathway was explored. Once dicarbonyl compounds were formed during the Maillard reaction, the addition of l ‐cysteine had no color‐inhibiting effect; if l ‐cysteine was added immediately after the Amadori compound was formed, the extraordinary color‐inhibiting effect was observed. Therefore, an improved way to inhibit color formation was proposed on the basis of the interaction of l ‐cysteine and Amadori compounds by controlling the addition time of l ‐cysteine through gradient temperature‐elevating Maillard reaction. The system was heated at 80 °C for 60 min to form Amadori compounds, followed by the addition of L‐cysteine, and the temperature was raised to 120 °C and held for 110 min. Compared with traditional products, the lightest color product was found desirable by GC/MS analysis and sensory evaluation. The novel method proposed can be a guide for the industrial preparation of light‐colored products. Copyright © 2012 European Peptide Society and John Wiley & Sons, Ltd.     

Covalent modification of subtilisin Bacillus lentus cysteine mutants with enantiomerically pure chiral auxiliaries causes remarkable changes in activity

Methanethiosulfonate reagents may be used to introduce virtually unlimited structural modifications in enzymes via reaction with the thiol group of cysteine. The covalent coupling of enantiomerically pure (R) and (S) chiral auxiliary methanethiosulfonate ligands to cysteine mutants of subtilisin Bacillus lentus induces spectacular changes in catalytic activity between diastereomeric enzymes. Amidase and esterase kinetic assays using a low substrate approximation were used to establish kcat/KM values for the chemically modified mutants, and up to 3-fold differences in activity were found between diastereomeric enzymes. Changing the length of the carbon chain linking the phenyl or benzyl oxazolidinone ligand to the mutant N62C by a methylene unit reverses which diastereomeric enzyme is more active. Similarly, changing from a phenyl to benzyl oxazolidinone ligand at S166C reverses which diastereomeric enzyme is more active. Chiral modifications at S166C and L217C give CMMs having both high esterase kcat/KM's and high esterase to amidase ratios with large differences between diastereomeric enzymes.     

Protein dolichylation in Plasmodium falciparum

We performed reverse-phase thin-layer chromatography and reverse-phase high-performance liquid chromatography (RP-HPLC) analysis of polyisoprenoids released by sulfonium-salt cleavage with methyl iodide from Plasmodium falciparum proteins labeled with [3H]FPP or [3H]GGPP and showed that a dolichol of 11 isoprene units is bound to 21-28-kDa protein clusters from trophozoite and schizont stages. The dolichol structure was confirmed by electrospray-ionization mass spectrometry analysis. Treatment with protein synthesis inhibitors and RP-HPLC analysis of the proteolytic digestion products from parasite proteins labeled with [35S]cysteine and [3H]FPP showed that the attachment of dolichol to protein is a post-translational event and probably occurs via a covalent bond to cysteine residues.     

Photocontrol of kinesin ATPase activity using an azobenzene derivative

Azobenzene is a photochromic molecule that undergoes rapid and reversible isomerization between the cis- and trans-forms in response to ultraviolet (UV) and visible (VIS) light irradiation, respectively. Here, we introduced the sulfhydryl-reactive azobenzene derivative 4-phenylazophenyl maleimide (PAM) into the functional region of kinesin to reversibly regulate the ATPase activity of kinesin by photoirradiation. We prepared five kinesin motor domain mutants, A247C, L249C, A252C, G272C and S275C, which contained a single reactive cysteine residue in loops L11 and L12. These loops are considered to be key regions for the functioning of kinesin as a motor protein. PAM was stoichiometrically incorporated into the cysteine residues in the loops of the mutants. The PAM-modified S275C mutant exhibited reversible alterations in ATPase activity accompanied by cis-trans isomerization upon UV and VIS light irradiation. The ATPase activity exhibited by the cis-isomer of the PAM bound to the mutant was two times higher than that of the trans-isomer. Further, the PAM-modified L249C mutant exhibited reversible alterations in ATPase activity on UV-VIS light irradiation but exhibited the opposite effect on UV and VIS light irradiation. Using a photochromic azobenzene derivative, we have demonstrated that the ATPase activity of the motor protein kinesin is photoregulated.     

海绵来源链霉菌S52-B中氨酰胺天然产物的分离与鉴定

【背景】海洋微生物是复杂海洋生态环境中重要的生物资源之一。海洋微生物所产生的活性天然产物极为丰富,是药物或药物先导化合物的重要来源。【目的】探索海洋中海绵来源链霉菌Streptomycessp.S52-B的优势生长条件,挖掘其次级代谢产物,以期分离具有良好生物活性的天然产物。【方法】根据"One Strain Many Compounds"(OSMAC)策略,寻找利于Streptomyces sp. S52-B生长和次级代谢产物产生的优势培养基,结合质谱及特征性的紫外吸收谱图,选择培养基进行大量发酵。利用正相硅胶柱色谱、葡聚糖凝胶柱色谱和制备型高效液相色谱等进行分离纯化,并应用高分辨质谱和核磁共振光谱进行化合物结构解析。【结果】确定培养基A–D为海洋链霉菌S52-B的优势培养基,基于紫外吸收光谱与质谱分析,从培养基A的大量发酵物中分离鉴定3个具有吡咯并[4,3,2-de]喹啉核心结构的含氯化合物,属于氨酰胺类天然产物,其中Ammosalic acid为新结构化合物。【结论】已知含有吡咯并喹啉母核的氨酰胺类家族化合物具有优良的抗癌活性。本研究从海绵来源链霉菌S52-B中分离鉴定了3个氨酰胺类化合物,其中一个是新结构化合物,不仅丰富了此类化合物家族的结构类型,也为研究其生物合成途径中的未知机理奠定了基础,还有利于结合培养条件和基因组信息从这株海绵来源链霉菌中挖掘新结构的活性天然产物。     

A temperature-sensitive mutant ofEscherichia coli with an alteration in ribosomal protein L22

A temperature-sensitive, protein synthesis-defective mutant ofEscherichia coli exhibiting an altered ribosomal protein L22 has been investigated. The temperature-sensitive mutation was mapped to therplV gene for protein L22. The genes from the wild type and mutant strains were amplified by the polymerase chain reaction and the products were sequenced. A cytosine to thymine transition at position 22 of the coding sequence was found in the mutant DNA, predicting an arginine to cysteine alteration in the protein. A single cysteine residue was found in the isolated mutant protein. This amino acid change accounts for the altered mobility of the mutant protein in two-dimensional gels and during reversed-phase HPLC. The temperature-sensitive phenotype was fully complemented by a plasmid carrying the wild type L22 gene. Ribosomes from the complemented cells showed only wild type protein L22 by two dimensional gel analysis and were as heat-resistant as control ribosomes in a translation assay. The point mutation in the L22 gene is uniquely responsible for the temperature-sensitivity of this strain.     

人EGF受体L2结构域在大肠杆菌中表达、包涵体柱上复性及纯化

以PCR方法从克隆的EGFR胞外区cDNA中扩增编码EGFR-L2结构域的DNA片段,在其3′端加入编码His6标签的序列,与pET-3c连接构建EGFR-L2原核表达载体。该蛋白在大肠杆菌BL21(DE3)中获得高效表达,免疫印迹分析表明表达产物全部以包涵体形式存在,分步透析法和稀释法都不能获得可溶性复性产物,而Ni²⁺-NTA柱上复性法不仅能够获得可溶性的EGFR-L2蛋白,而且产物同时得到高度纯化,纯度>95％,复性的EGFR-L2与其配基EGF具有特异性的结合活性,但亲和力较低。这表明His6标签不但便于纯化目标蛋白,而且可利用Ni²⁺-NTA柱进行柱上复性,适用于不易通过常规方法复性的重组蛋白的制备。     

Synthesis and luminescence properties of 2‐(benzylcarbamoyl)phenyl derivatives and their europium complexes

Six novel 2‐(benzylcarbamoyl)phenyl derivatives were synthesized and characterized by ¹H‐NMR, mass spectrometry, infrared spectra and elemental analysis. Their europium complexes were prepared and characterized by elemental analysis, EDTA titrimetric analysis, IR and UV spectra as well as molar conductivity measurements. The luminescence properties of these complexes were investigated and results show that 2‐(benzylcarbamoyl)phenyl derivatives possess high selectivity and good coordination with the europium ion. Complex Eu‐2‐(benzylcarbamoyl)phenyl‐2‐phenylacetate showed green luminescence that was emitted by the ligand of 2‐(benzylcarbamoyl)phenyl‐2‐phenylacetate, while other complexes showed the characteristic red luminescence of europium ion and also possessed high luminescence intensity. Copyright © 2012 John Wiley & Sons, Ltd.