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二酪氨酸:制备、分离及分析

Dityrosine: preparation, isolation, and analysis.

作者信息

Malencik D A, Sprouse J F, Swanson C A, Anderson S R

机构信息

Department of Biochemistry and Biophysics, Oregon State University, Corvallis 97331, USA.

出版信息

Anal Biochem. 1996 Nov 15;242(2):202-13. doi: 10.1006/abio.1996.0454.

Abstract

This article describes chromatographic and spectroscopic techniques that have multiple applications in the preparation, isolation, and analysis of dityrosine. A three-step chromatographic procedure facilitates the preparation of 120 mg or more (yield > 26% of theoretical maximum) of dityrosine from the enzyme-catalyzed oxidation of tyrosine. DEAE-cellulose chromatography performed in a boric acid-sodium borate buffer removes most of the contaminating pigments. Two-dimensional pH-dependent chromatography on BioGel P-2 separates dityrosine from tyrosine, residual pigments, salts, etc. Elemental analysis indicates that the purified product is approximately 92% dityrosine by weight. Fast atom bombardment mass spectrometry and two types of reverse-phase high-performance liquid chromatography (HPLC), monitored in fluorescence and absorbance measurements, verify the purity of the dityrosine. The distinctive pH-dependent chromatography of dityrosine on BioGel P-2, with reversible adsorption to the matrix occurring at pH values less than 3, is useful for the isolation of varying quantities of dityrosine and for analysis per se. Affinity chromatography on immobilized phenyl boronate (Matrex Gel PBA-60) is an alternate method for the isolation and determination of dityrosine, which undergoes specific interactions with the boronate moiety and possible hydrophobic association with the phenyl group. Two new reverse-phase HPLC techniques expedite the analysis of picomole quantities of dityrosine. One employs isocratic elution (92% H2O, 8% acetonitrile, and 0.1% trifluoroacetic acid) of an ODS II Spherisorb column, with both fluorometric and spectrophotometric detection. The other procedure may be performed in conjunction with total amino acid analysis. A rapid gradient program, developed with a Phenomenex Ultracarb 20 column, clearly separates dabsylated dityrosine and tyrosine from other dabsylated amino acids. It is especially useful when dityrosine is a trace component.

摘要

本文介绍了在二酪氨酸的制备、分离和分析中具有多种应用的色谱和光谱技术。一种三步色谱法有助于从酪氨酸的酶促氧化反应中制备120毫克或更多的二酪氨酸(产率>理论最大值的26%)。在硼酸 - 硼酸钠缓冲液中进行的DEAE - 纤维素色谱法可去除大部分污染色素。在BioGel P - 2上进行的二维pH依赖性色谱法可将二酪氨酸与酪氨酸、残留色素、盐等分离。元素分析表明,纯化产物按重量计约为92%的二酪氨酸。快速原子轰击质谱法和两种通过荧光和吸光度测量监测的反相高效液相色谱(HPLC)法,验证了二酪氨酸的纯度。二酪氨酸在BioGel P - 2上独特的pH依赖性色谱法,在pH值小于3时会与基质发生可逆吸附,这对于分离不同量的二酪氨酸及其本身的分析很有用。固定化苯基硼酸(Matrex Gel PBA - 60)上的亲和色谱法是分离和测定二酪氨酸的另一种方法,二酪氨酸与硼酸部分发生特异性相互作用,并可能与苯基发生疏水缔合。两种新的反相HPLC技术加快了对皮摩尔量二酪氨酸的分析。一种方法采用ODS II Spherisorb柱的等度洗脱(92%水、8%乙腈和0.1%三氟乙酸),同时进行荧光和分光光度检测。另一种方法可与总氨基酸分析一起进行。用Phenomenex Ultracarb 20柱开发的快速梯度程序可将二甲基氨基苯磺酰化的二酪氨酸和酪氨酸与其他二甲基氨基苯磺酰化的氨基酸清晰分离。当二酪氨酸是痕量成分时,它特别有用。

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