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基于固体载体的果胶低聚半乳糖醛酸酶促合成及其基质辅助激光解吸电离飞行时间质谱分析

Solid-supported enzymatic synthesis of pectic oligogalacturonides and their analysis by MALDI-TOF mass spectrometry.

作者信息

Guillaumie Fanny, Sterling Jason D, Jensen Knud J, Thomas Owen R T, Mohnen Debra

机构信息

Center for Process Biotechnology, BioCentrum-DTU, Technical University of Denmark, Building 223, Søltofts Plads, DK-2800 Kgs Lyngby, Denmark.

出版信息

Carbohydr Res. 2003 Sep 10;338(19):1951-60. doi: 10.1016/s0008-6215(03)00321-5.

DOI:10.1016/s0008-6215(03)00321-5
PMID:14499571
Abstract

Solid-phase biosynthetic reactions, followed by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry analysis (MALDI-TOF), was used to gain insight into the biosynthesis of pectin oligomers. Sepharose supports bearing long pectic oligogalacturonides (OGAs) anchored through a disulfide-containing cleavable linker, were prepared. The OGAs (degrees of polymerization of 13 and 14) were efficiently immobilized through the reducing end via formation of an oxime linkage. These OGA-derivatized matrices were subsequently employed in novel solid-phase enzymatic reactions, with the pectin biosynthetic enzyme, alpha-1,4-galacturonosyltransferase, GalAT (solubilized from Arabidopsis thaliana) and the glycosyl donor, uridine diphosphate-galacturonic acid (UDP-GalA). Solid-supported biosynthesis was followed by cleavage of the immobilized OGAs and direct analysis of the products released into the liquid phases by MALDI-TOF mass spectrometry. In time course studies conducted with an immobilized (alpha-D-GalA)14 and limiting amounts of the glycosyl donor, the predominant product was an OGA extended by one GalA residue at the non-reducing end (i.e., (GalA)15). When UDP-GalA was added in approximately excess compared to immobilized (GalA)13, OGAs up to the 16-mer were synthesized, confirming the non-processivity of the GalAT in vitro.

摘要

采用固相生物合成反应,随后进行基质辅助激光解吸/电离飞行时间质谱分析(MALDI-TOF),以深入了解果胶寡聚物的生物合成过程。制备了通过含二硫键的可裂解连接子固定有长果胶低聚半乳糖醛酸(OGAs)的琼脂糖载体。通过形成肟键,OGAs(聚合度为13和14)通过还原端有效地固定化。这些OGA衍生化的基质随后用于新型固相酶促反应,使用果胶生物合成酶α-1,4-半乳糖醛酸转移酶GalAT(从拟南芥中溶解)和糖基供体尿苷二磷酸-半乳糖醛酸(UDP-GalA)。固相支持的生物合成之后是固定化OGAs的裂解,并通过MALDI-TOF质谱直接分析释放到液相中的产物。在用固定化的(α-D-GalA)14和限量的糖基供体进行的时间进程研究中,主要产物是在非还原端延伸一个GalA残基的OGA(即(GalA)15)。当与固定化的(GalA)13相比加入大约过量的UDP-GalA时,合成了直至16聚体的OGAs,证实了GalAT在体外的非持续性。

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