亚甲基蓝褪色光度法测定肝素

用紫外-可见光谱法研究肝素(Hep)对亚甲基蓝(MB)的褪色反应,在pH3.0的BrittonRobinson缓冲溶液中,肝素与亚甲基蓝形成离子缔合物时,染料发生明显的褪色,体系吸光度的降低与肝素钠浓度成正比.建立了一种简单、灵敏、选择性高的肝素测定方法.本法在0-4.0μg/mL范围内呈现良好的线性关系(r=0.9978),回收率范围为98.8%-101.9%.用于肝素钠注射液的分析,结果令人满意.     

碱性二苯基萘基甲烷染料褪色分光光度法测定肝素

肝素(Heparin, Hep)由葡萄糖胺磺酸、葡萄糖醛酸和艾杜糖醛酸组成, 在水溶液中由于其酸性基团的离解而成为带多个负电荷的大阴离子[1].肝素具有广泛的生物学功能, 在人体内由肥大细胞分泌而自然存在于血液中, 在体内外均有延缓或阻止血液凝固的作用. 肝素或其衍生物还可用于调血脂、抗血栓、改善血液流变学指标、抗炎、抗过敏及免疫调节等, 是重要的生化药物之一 [2]. 对不同的疾病, 肝素有不同的最适剂量, 临床上常采用生物方法 [3]来进行监控. 但由于受生物个体的影响较大, 故使其应用受到限制. 此外, 分光光度法 [1,4,5]、荧光法[6]、HPLC法[7]、细管电泳法[8]及电化学传感器[9]已用于肝素的测定, 其中分光光度法由于操作简便、快速、仪器价廉和灵敏度较高等优点而得到重视.     

Separation, identification, and interaction of heparin oligosaccharides with granulocyte-colony stimulating factor using capillary electrophoresis and mass spectrometry

A capillary electrophoresis (CE) method was developed for the separation of heparin oligosaccharides compatible to study the interactions between the oligosaccharides and granulocyte-colony stimulating factor (G-CSF). Unfractionated heparin was eliminitively degraded to heparin oligosaccharides by an endolytic heparinase. The degraded smaller oligosaccharides (M(r) < 1000) were baseline-separated by CE under a 50 mM phosphate buffer (pH 9.0) in 10 min. Standard heparin disaccharides and larger oligosaccharides (1000 < M(r) < 8000) were all separated under optimized separation conditions. Compared with standard heparin disaccharides, smaller oligosaccharides contained one nonsulfated, two monosulfated, and two disulfated disaccharides, but trisulfated disaccharides were not found. The smaller oligosaccharides were also identified and molecular mass was deduced by electrospray ionization-mass spectrometry (ESI-MS). Furthermore, interactions between G-CSF and the oligosaccharides were studied by using capillary zone electrophoresis (CZE) under the above separation conditions. It was found that larger oligosaccharides could interact with G-CSF while smaller oligosaccharides were not observed to bind to G-CSF under the experimental conditions. In conclusion, the purified heparinase could selectively degrade heparin into oligosaccharides and the interaction between G-CSF and heparin was correlated with the chain length of heparin.     

Preparation of a set of selectively protected disaccharides for modular synthesis of heparan sulfate fragments: toward the synthesis of several <Emphasis Type="Italic">O</Emphasis>-sulfonated [β-D-GlcUA-(1→4)-β-D-GlcNAc]OPr types

A concise method for a stereocontrolled synthesis of a set of selectively protected disaccharides is reported. Coupling of the donor 11 onto acceptors 23 and 24, promoted by trimethylsilyl triflate-N-iodosuccinimide (TMSOTf-NIS), generated the disaccharides 25 and 26. Under typical conditions, condensation of the fully protected donor 12 onto acceptors 23 and 24 produced the disaccharides 27 and 28. The building blocks 25–28 were prepared in moderate yields having exclusive β-stereoselectivity. A unique pattern of protecting groups distinguished clearly between positions to be sulfated and functional groups remaining as free hydroxyl groups. Acetyl and/or levulinoyl esters temporarily protected the positions to be sulfated, while benzyl ethers were used for permanent protection. The anomeric positions were protected as allyl ethers, whereas the 4′-positions were masked as p-methoxybenzyl (PMB) ethers. The orthogonality of the PMB and allyl groups can then be used for further elongation of the chain by recurrent deprotection and activation steps. The hydroxyl group, OH-6, of glucosamine moieties was protected as a TBDPS ether to avoid oxidation. A five-step deprotection/sulfonation sequence was applied to the disaccharide 27 to generate the corresponding sulfated [β-D-GlcUA-2-OSO₃Na-(1→4)-β-D-Glc pNAc]-(1→O-Pro) 34.     

肝素化聚甲基硅氧烷-聚氧乙烯接枝物的合成及其体外抗凝血性能评价

以二甲基硅油接枝端羟基聚氧乙烯（ＰＤＭＳ ｇ ＰＥＯ ＯＨ）为基材，用二环己基碳二亚胺（ＤＣＣＩ）作脱剂，研究了羟基（ＯＨ）与肝素上的羧基（—ＣＯＯＨ）之间的脱水缩合反应，制备出肝素化的抗血栓材料ＰＤＭＳ ｇ ＰＥＯ Ｈｅｐ，并对其涂覆表面的肝素含量和体外抗凝血性能进行了初步评价．实验结果表明，肝素接枝的共聚物具有优良的抗凝血性能和一定的应用前景．     

硫堇褪色光度法测定微量肝素

在pH 4.10的Britton-Robinson缓冲溶液中,肝素与碱性吩噻嗪染料硫堇形成离子缔合物时,染料发生明显的褪色。体系吸光度的降低与肝素钠浓度成正比,肝素的质量浓度在0~60μg/25 mL范围内符合比耳定律,摩尔吸光系数为3.58×106L.mol-1.cm-1。研究了表面活性剂和共存物质的影响,表明方法选择性好。用于肝素钠注射液效价的测定,相对标准偏差小于3%,回收率为96.5%~101.9%。     

Amperometry of Heparin Polyion Using a Rotating Disk Electrode Coated with a Plasticized PVC Membrane

Electrochemical method of detection of heparin polyion was developed based on voltammetry of heparin on a rotating glassy carbon (GC) electrode coated with a plasticized PVC membrane. The membrane was deposited on the GC disk by spin‐coating technique using a mixture of solutions of PVC in tetrahydrofuran, and 1,1′‐dimethylferrocene (DMFc) and hexadecyltrimethylammonium tetrakis(4‐chlorophenyl)borate (HTMATPBCl) in o‐nitrophenyl octyl ether. UV/vis reflection spectrometry was used to evaluate the membrane thickness, which exhibits a linear correlation with the membrane resistance measured by impedance spectroscopy. It is shown that this electrode can be used for amperometric or coulometric detection of heparin in aqueous samples of medically relevant concentrations (1–10 U mL^?1), with a detection limit of 1.4 U mL^?1. Evidence is provided indicating that the current determining step is the reversible adsorption of the ion‐pair of heparin polyion with HTMA⁺ cation at the membrane/aqueous electrolyte interface, which is driven by oxidation of DMFc at the GC/membrane interface.     

Spectrophotometric and Voltammetric Studies on the Interaction of Heparin with Phenosafranine

The interaction of phenosafranine （PSF） with a glycosaminoglycans of heparin （Hep） in aqueous solution has been characterized by UV-Vis absorption spectrophotometry and cyclic voltammetry in pH 1.5 Britton-Robinson （B-R） buffer solution. The addition of Hep caused decrease of the absorbance of PSF at 532 nm and the redox peak current of PSF. The study showed that an supramolecular complex of PSF-Hep was formed because of the electrostatic attraction of negatively charged Hep with the positively charged PSF, which resulted in the decrease of the equilibrium concentration of PSF in solutions, and the decrease of the absorbance or the peak current of PSF. The stoichiometry of the Hep/PSF complex was further calculated by voltammetric data with the result of 1：1 complex.     

Relative retention of the fibroblast growth factors FGF-1 and FGF-2 on strong cation-exchange sorbents

The isocratic retention of two heparin-binding fibroblast growth factors, FGF-1 (acidic FGF) and FGF-2 (basic FGF), was compared on a set of six preparative strong cation-exchange adsorbents. The FGFs comprise a solute pair that are structurally equivalent, yet differ in protein parameters of potential importance in cation-exchange chromatography, such as isoelectric point, net charge, and the number and distribution of basic amino acids. The cation-exchange adsorbents comprise a diverse set of materials in common use for protein purification, with physical and chemical properties that have been characterized and described previously. Isocratic k' values for the two proteins obtained on each adsorbent at several different [NaCl] are compared with one another and with corresponding data for hen egg lysozyme, which is also strongly retained on cation-exchangers. Of the six adsorbents examined, three showed strong retention of both FGFs, with equivalent k' values for FGF-1 and FGF-2. Three others, which showed weaker overall retention for the FGF pair, showed much larger retention differences between FGF-1 and FGF-2. The trends in retention order among the stationary phases are very similar to those seen previously with other unrelated proteins. However, retention differences between the two FGFs, and between the FGFs and lysozyme, do not correlate well with simple charge properties such as net charge, indicating, as in some previous studies, the importance of local regions on the protein surface in determining retention. These observations are interpreted in terms of the structural features of the proteins and the physicochemical properties of the adsorbents.     

Resonance Rayleigh scattering, frequency doubling scattering and second-order scattering spectra of the heparin-crystal violet system and their analytical application

In pH 6.0-11.2 Britton-Robinson buffer solution, binding of heparin with crystal violet (CV) can result in a significant enhancement of resonance Rayleigh scattering (RRS) and resonance non-linear scattering, such as frequency doubling scattering (FDS) and second-order scattering (SOS). Their maximum scattering wavelengths, λ_ex/λ_em, appear at 492 nm/492 nm for RRS, 984 nm/492 nm for FDS and 492 nm/984 nm for SOS, respectively. The optimum conditions of the reaction, the influencing factors and the relationship between the three scattering intensities and the concentration of heparin have been investigated. New methods for the determination of trace amounts of heparin based on the RRS, FDS and SOS methods have been developed. The methods exhibit high sensitivities, the detection limit for heparin is 2.9 ng ml⁻¹ for the RRS method, 3.5 ng ml⁻¹ for the FDS method and 3.3 ng ml⁻¹ for the SOS method. The methods have good selectivity and were applied to the determination of heparin in heparin sodium injection samples with satisfactory results.