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1.
《Angewandte Chemie (Weinheim an der Bergstrasse, Germany)》2017,129(38):11578-11583
The thermoresponsive behavior of an elastin‐based polymer can be altered by the polymeric macromolecular conformation. Thus, when the elastin basic amino acid sequence VPGVG is used as a pendant group of a poly(phenylacetylene) (PPA) its thermoresponsive behavior in water can be remotely detected through conformational changes on the formed helix. Circular dichroism at different temperatures shows an inversion of the first Cotton effect (450 nm) at 25.8 °C that matches with the cloud point temperature. The elastin‐based side‐chain poly(phenylacetylene) shows an upper critical solution temperature with low pH and concentration dependency, not expected in elastin‐based polymers. It was found that the polymer self‐assembles in water into spherical nanoparticles with hydrodynamic diameters of 140 nm at the hydrophobic state. 相似文献
2.
Sionkowska A Skopinska J Wisniewski M Leznicki A 《Journal of photochemistry and photobiology. B, Biology》2007,86(2):186-191
An investigation into the influence of UV irradiation on elastin hydrolysates in the presence of collagen was carried out using UV-Vis spectroscopy and spectrofluorometry. It was found that the absorbance of elastin hydrolysates in solution increased during irradiation more than the absorbance of the elastin/collagen blend. The fluorescence of elastin hydrolysates was observed at 305nm and at 380nm after excitation at 270nm. For the elastin/collagen mixture in solution, fluorescence spectrum shows only one maximum at 305nm. UV irradiation caused fluorescence fading at 305nm. For irradiated elastin the fluorescence at 305nm decreased faster than for the irradiated elastin/collagen mixture. The maximum of the fluorescence peak was shifted for elastin by 4nm, whereas for the elastin/collagen blends the shift was only 1-2nm. All the obtained results point out the ability of mixing elastin and collagen, and suggest that the elastin/collagen mixture in solution is less sensitive to UV irradiation than elastin hydrolysates alone. 相似文献
3.
4.
Sionkowska A Skopinska J Wisniewski M Leznicki A Fisz J 《Journal of photochemistry and photobiology. B, Biology》2006,85(1):79-84
An investigation into the influence of UV irradiation on elastin hydrolysates dissolved in water was carried out using UV-Vis spectroscopy and spectrofluorometry. It was found that the absorption of elastin hydrolysates in solution increased during irradiation of the sample. For fluorescence of elastin hydrolysates we observed both, a decrease and increase of this value during irradiation of the sample. After UV irradiation of the elastin solution we observed a minor increase of overall absorption, most notably between 250 nm and 280 nm. Moreover, after UV irradiation a wide peak emerged between 290 nm and 310 nm with maximum at about 305 nm. The new peak suggests that new photoproducts are formed during UV irradiation of elastin hydrolysates. The fluorescence of elastin hydrolysates was observed at 305 nm and at 380 nm after excitation at 270 nm. UV irradiation caused fluorescence fading at 305 nm and 380 nm. After 30 min of irradiation a new broad weak band of fluorescence, attributable to new photoproducts, emerged in the UV wavelength region with emission maximum between 400 nm and 500 nm. 相似文献
5.
灵芝发酵液中蛋白酶抑制剂GLPIA2的纯化及其特性 总被引:1,自引:0,他引:1
采用乙醇分级沉淀、凝胶色谱纯化、阴离子交换色谱分离等步骤从灵芝深层发酵液中提取得到蛋白酶抑制剂GLPIA1
与GLPIA2。其中GLPIA2仅在215 nm处有紫外吸收,经十二烷基硫酸钠-聚丙烯酰胺凝胶电泳鉴定为单一条带,相对分子质
量为15000。由其氨基酸组成分析谱图可看出,其酸性氨基酸含量较高,碱性氨基酸及芳香族氨基酸含量较低。GLPIA2抑
制剂的底物特异性研究表明,它对天冬氨酸族的胃蛋白酶和酵母蛋白酶A有相对较强的抑制作用。 相似文献
6.
A sensitive chromatographic determination of hydrazines by naphthalene-2,3-dialdehyde derivatization
Alexander D. Smolenkov Alla V. Chernobrovkina Roman S. Smirnov Mikhail G. Chernobrovkin Oleg A. Shpigun 《International journal of environmental analytical chemistry》2013,93(12):1286-1295
A new high-performance liquid chromatography (HPLC) method for the sensitive simultaneous determination of hydrazine (Hy), monomethylhydrazine (MMH) and 1,1-dimethylhydrazine (UDMH) based upon the derivatization of hydrazines with naphthalene-2,3-dialdehyde and the separation of the derivatives on Zorbax Eclipse AAA column in a single chromatographic run under acidic conditions (pH 2.4) was developed. Hydrazine and monomethylhydrazine derivatives were found to be strongly fluorescent at λex?=?273?nm, λem?=?500?nm. It was shown that UDMH derivative can be detected as non-fluorescent hydrazone at 290?nm by UV-detection. Limits of detection were 0.05?µg?·?L?1 for Hy and MMH, and 1?µg?·?L?1 for UDMH for the injection volume of 100?µL. The method was validated for water sample analysis. It proved to be selective, accurate and precise with the supplementary advantage of the simple and rapid sample preparation. 相似文献
7.
The solubilization of human lung elastin by leucocyte elastase and cathepsin G is described. Elastolysis kinetic studies clearly show that leucocyte elastase is more efficient in solubilizing elastin fibres than is cathepsin G. Cathepsin G can degrade elastin but at a much slower rate. Characterization of elastase and cathepsin G soluble elastin fragments, obtained after 24 h of digestion (enzyme-substrate ratio, 1:100), was first performed by isoelectric focusing. Whole digests were focused as 6 bands in a pH range 4.2 to 4.7 and were found to have no significant differences in amino acid compositions. Biogel P-100 gel filtration of the elastase digested fragments separated a major excluded fraction (Mr's: 80,000 to 30,000) and a small retained one (Mr's: 6000 to 4000). Conversely, cathepsin G digests were eluted as a minor excluded fraction and a more important retarded one (Mr's: 6000 to 4000). Only the high molecular weight fractions of both enzymes digests contain crosslinked amino acids; this assigns a role for desmosines in the resistance of elastin to these proteases. These results are discussed in comparison with the data obtained by others. 相似文献
8.
Laura Marcu Warren S. Grundfest Jean-Michel I. Maarek 《Photochemistry and photobiology》1999,69(6):713-721
To study the photobleaching of the main fluorescent compounds of the arterial wall, we repeatedly measured the time-resolved fluorescence of elastin, collagen and cholesterol during 560 s of excitation with nitrogen laser pulses. Three fluence rate levels were used: 0.72, 7.25 and 21.75 microW/mm2. The irradiation-related changes of the fluorescence intensity and of the time-resolved fluorescence decay constants were characterized for the emission at 390, 430 and 470 nm. The fluorescence intensity at 390 nm decreased by 25-35% when the fluence delivered was 4 mJ/mm2, a common value in fluorescence studies of the arterial wall. Cholesterol fluorescence photobleached the most, and elastin fluorescence photobleached the least. Photobleaching was most intense at 390 nm and least intense at 470 nm such that the emission spectra of the three compounds were markedly distorted by photobleaching. The time-resolved decay constants and the fluorescence lifetime were not altered by irradiation when the fluence was below 4 mJ/mm2. The spectral distortions associated with photobleaching complicate the interpretation of arterial wall fluorescence in terms of tissue content in elastin, collagen and cholesterol. Use of the time-dependent features of the emission that are not altered by photobleaching should increase the accuracy of arterial wall analysis by fluorescence spectroscopy. 相似文献
9.
Israel S. Ibarra Karina Aguilar-Arteaga Elizabeth Contreras-Lopez Enrique Barrado 《Analytical letters》2013,46(11):1732-1742
A magnetic separation method based on the use of magnetic silica as the stationary phase in sequential injection chromatography was used for simultaneous determination of nonsteroidal anti-inflammatory drugs (acetaminophen, naproxen, diclofenac, and ibuprofen) in tablets. The method is based on a thin layer paramagnetic stationary phase retained on the inner wall of a mini-column through the action of an external magnetic field. The influence of the variables involved was evaluated and the optimal conditions were found to be: a methyl-silica magnetic adsorbent was used as the stationary phase, the mobile phase was methanol-water (60:40, v/v), pH 2.5 adjusted with 98% phosphoric acid, a flow rate 0.60 ml min?1, and UV detection at 225 nm. Under these conditions, the linear range of the calibration curve ranged from 3–6 mg L?1 to 100 mg L?1 with limits of detection ranging between 1 to 2 mg L?1. The proposed method was validated by comparing the results obtained against those provided by high performance liquid chromatography; no significant differences were seen. 相似文献
10.
Philippe Giummelly Bernard Botton Raphaë lle Friot Deddi Prima-Putra Jeffrey Atkinson 《Journal of chromatography. A》1995,710(2):357-360
Desmosine (DES) and isodesmosine (IDE) were separated and quantitated by a simple and sensitive capillary zone electrophoretic (CZE) method, using hydrostatic injection and direct UV detection at 254 or 185 nm. Two different electrophoretic mobilities for the two isoforms were observed in 90 mM phosphoric acid pH 2.2. The presence of a mixture of amino acids in the sample did not affect the separation of DES and IDE. The method was successfully used to quantitate the amounts of DES and IDE in elastin hydrolysates. 相似文献
11.
Animal fibrous proteins (AFPs) such as egg-shell membrane (ESM), chicken feather (CF), wool, silk, or elastin are an intricate
network of stable and water-insoluble fibers with high surface area and are abundant bioresources. Every AFP tested was found
to accumulate gold-cyanide ion from aqueous solutions in high yield, depending on pH and some other parameters. Gold-cyanide
ion is adsorbed by AFP at low pH range, with maximum binding observed at approx pH 2.0. Under the certain conditions, gold-cyanide
ion was accumulated up to 8.6, 7.1, 9.8, 2.4, and 3.9% of dry weight on ESM, CF, wool, silk, and elastin, respectively. In
the case of ESM, it was found that ESM removed gold-cyanide ion almost quantitatively and almost all the gold uptake by ESM
was easily desorbed with 0.1M NaOH. ESM can be used repeatedly for the process of gold adsorption-desorption. The gold-biosorptive capacity of ESM that
was chemically modified with glutaraldehyde was higher than that of control. In column procedure, ESM packed on column removed
gold-cyanide ion from the dilute aqueous solution to extremely low concentrations (nondetectable concentration of below 1
ppb) 相似文献
12.
采用超滤浓缩、强阴离子交换、疏水作用和凝胶色谱等方法, 对毕赤酵母表达的rGlip进行分离和纯化, 对离子交换色谱中rGlip与固相结合的最佳pH值进行了考察, 并对纯化产物的活性进行了鉴定. rGlip在215 nm处有强的紫外吸收, 经激光解析电离时间飞行质谱鉴定其相对分子量为12722, 经反相液相色谱鉴定纯度≥97%. 设计rGlip的疏水作用色谱, 有效地去除色素. 凝血实验结果表明, rGlip可以凝集绵羊血红细胞, 但对人血A, B, AB和O型等红细胞无凝集作用, 有类似凝集素的生物学活性. 相似文献
13.
建立了用阴离子交换色谱法测定小球藻提取物中的各种核苷酸的方法。用Shim PackWAX 1色谱柱 (5 0mm× 4 .6mmi.d .,粒度 3μm ,孔径 1 0 0nm) ,2 5mmol/L的磷酸二氢钠水溶液 (pH =3.5 ) ,流量梯度洗脱。检测波长 2 6 0nm。回收率在 97.5 0 %~ 99.4 0 %。该法简便 ,灵敏 ,重现性好 ,可以广泛应用于各类小球藻提取物和各类食品中的核苷酸的检测 相似文献
14.
反相离子对高效液相色谱法测定动物血浆中的恩诺沙星 总被引:2,自引:0,他引:2
1 前言恩诺沙星 ( enrofloxacin,ERFX)系全合成新一代喹诺酮类抗菌药、具有高效、广谱 ,耐药菌极少、副作用小等优点 ,是当今世界动物用最佳的抗感染类药物之一[1~ 5] 。Kung等[3] 认为 ERFX抗菌是其在体内代谢为环丙沙星 ( ciprofloxacin,CPFX)而发挥作用的。有关分析 ERFX文献较少[2 ] 。为了研究 ERFX的药代动力学 ,本文建立了 ERFX测定的反相离子对 HPLC分析方法。2 实验部分2 .1 仪器与试剂日本岛津 LC-6A高效液相色谱系统 ,具CTO-6A柱箱、SCL -6A系统控制器、SPD-6AV紫外 -可见检测器和 C-R3 A色谱数据处理机… 相似文献
15.
A method has been developed for the separation and quantitation of desmosines in tissue samples. The tissue is treated with cold 10% trichloroacetic acid to remove collagen and hydrolysed in HCl vapours in sealed vials. Preseparation of desmosines from tissue acid hydrolysates is performed on a cellulose column, first eluted with n-butanol-acetic acid-water to wash out other amino acids and then with water to recover desmosines. Separated desmosines are then derivatized with phenylisothiocyanate and determined by reversed-phase high-performance liquid chromatography using a gradient system with sodium acetate pH 6.4 and acetonitrile. Desmosines were detected spectrophotometrically at 254 nm. The method was applied to the determination of desmosine in elastin, rat aorta and bovine ligamentum nuchae. 相似文献
16.
HPLC-MS and MECC analysis of coumarins 总被引:4,自引:0,他引:4
Summary MECC separation of 11 coumarins has been achieved by use of a running electrolyte at pH 10.4 prepared from 50 mM boric acid,
10 mM sodium tetraborate and 100 mM sodium hydroxide. The buffer solution contained 50 mM SDS and, as organic modifier 1%n-propanol. The applied voltage was 25 kV and the temperature of the capillary was kept constant at 20°C. HPLC baseline separation
of the coumarin mixture was obtained by use of a reversed-phase column and an acetonitrile-water solvent gradient. UV detection
was performed at 205 nm. Peak assignment and purity control were achieved by HPLC-mass spectrometry with either an electrospray
interface or an atmospheric-pressure chemical-ionization interface. Compounds were detected in either negative- or positive-ion
modes. These MECC and HPLC-MS methods are suitable for ‘fingerprint’ analysis of a number of coumarin-containing plants, e.g.
Fr.Ammi visnagae, Rd.Scopoliae and Rd.Imperatoriae. 相似文献
17.
M. Freney H. Irth H. Lindberg U. Alkner L. Greiff C. G. A. Persson M. Andersson G. Marko-Varga 《Chromatographia》2001,54(7-8):439-445
Summary Fucose (6-deoxygalactose) is a constituent of airway mucous glycoproteins. In this paper we describe a high-throughput method
for screening nasal lavage fluid samples and induced sputum samples for fucose. Fucose was released by hydrolysis with 0.5m sulfuric acid at 100°C for 4 h. After pH adjustment remaining proteins were removed by on-line dialysis. Chromatography was
performed with two 300 mm×7.8 mm i.d. Bio-Rad Aminex HPX-87H columns arranged in a box-car configuration. Post-column derivatization
was performed with benzamidine under alkaline conditions. Fluorescence was monitored at an excitation wavelength of 360 nm,
using an optical cut-off filter of 420 nm. The limit of quantitation for fucose was 40 μm (S/N=3) in 300μL nasal lavage medium, with use of a 20-μL injection loop. Relative standard deviation (RSD) values for intra and inter assay data were below 15% and 20%, respectively, at spike levels of 635 μm l-fucose. The method was used to monitor the fucose content of human airway secretions.
Presented at: 23rd International Symposium on Chromatography, London, UK, October 1–5, 2000 相似文献
18.
高效液相色谱法测定南瓜粉中的4-氨基丁酸 总被引:15,自引:0,他引:15
采用强阳离子交换柱分离 ,pH梯度洗脱 ,邻苯二甲醛 (OPA)柱后衍生 ,荧光λex=338nm ,λem=42 5nm检测的高效液相色谱法测定了南瓜粉中的 4 氨基丁酸 (GABA)。若以GABA的峰高Y(μV)对进样质量X(μg)进行线性回归 ,则线性方程为Y =45 6 6X +1396 ,r =0 9998;GABA的平均回收率 (n =3)为 99%。方法稳定、快速、灵敏、准确。 相似文献
19.
A rapid and reliable method based on micellar electrokinetic capillary chromatography has been developed for the determination
of dexamethasone in cosmetics. Effects of buffer composition, concentration and pH, the detection wavelength, separation voltage,
and injection time were systematically investigated. The optimum conditions were: 30 mM borax buffer containing 20 mM sodium
dodecyl sulfate at pH 9.0, detection at 254 nm, injection time 10 s at a height of 10 cm, and a separation voltage of 15 kV.
Under these conditions, the analysis of dexamethasone in cosmetics was carried out within 6 min. The method was validated
for stability, precision, linearity and accuracy. Excellent linearity was obtained in the range of 50–1,000 μg mL−1, and acceptable precision, in intra-day and inter-day analysis, was also obtained with relative standard deviation in the
range of 0.19–0.86 and 2.50–4.90% for migration time and peak area ratio, respectively. The method was used to analyse eight
cosmetic samples purchased locally. 相似文献
20.
Time-resolved fluorescence spectra of arterial fluorescent compounds: reconstruction with the Laguerre expansion technique 总被引:2,自引:0,他引:2
The time-resolved fluorescence spectra of the main arterial fluorescent compounds were retrieved using a new algorithm based on the Laguerre expansion of kernels technique. Samples of elastin, collagen and cholesterol were excited with a pulsed nitrogen laser and the emission was measured at 29 discrete wavelengths between 370 and 510 nm. The expansion of the fluorescence impulse response function on the Laguerre basis of functions was optimized to reproduce the observed fluorescence emission. Collagen lifetime (5.3 ns at 390 nm) was substantially larger than that of elastin (2.3 ns) and cholesterol (1.3 ns). Two decay components were identified in the emission decay of the compounds. For collagen, the decay components were markedly wavelength dependent and hydration dependent such that the emission decay became shorter at higher emission wavelengths and with hydration. The decay characteristics of elastin and cholesterol were relatively unchanged with wavelength and with hydration. The observed variations in the time-resolved spectra of elastin, collagen and cholesterol were consistent with the existence of several fluorophores with different emission characteristics. Because the compounds are present in different proportions in healthy and atherosclerotic arterial walls, characteristic differences in their time-resolved emission spectra could be exploited to assess optically the severity of atherosclerotic lesions. 相似文献