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ESI-MS and MALLS analysis of quaternary structure of molluscan hemocyanins

机译:软体动物血蓝蛋白季结构的ESI-MS和MALLS分析

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The understanding of the function of macromolecular complexes is mainly related to a precise knowledge of their structure. Recently, the development of suitable mass spectrometric techniques (electrospray ionization (ESI) and matrix-assisted laser desorption/ionization (MALDI)) and multi-angle laser light scattering has enabled mass determination of native complexes and of their subunits. By these techniques, the structure and association/dissociation behavior of huge molecules of molluscan Octopus vulgaris, Sepia officinalis and Rapana venosa have been characterized. Molecular masses of the native and dissociated molecule of cephalopodan Hcs O. vulgaris (3545 and 359.3 kDa, respectively) and S. officinalis (4134 and 443.8 kDa, respectively) revealed that only one type subunit organizes their molecules, while the presence of two isoforms with different masses (422.8 and 400.0 kDa) has been determined for gastropodan R. venosa Hc, aggregated into didecamers. The difference of their structural subunits was also established after limited proteolysis with TPCK-trypsin. Eight functional units (FUs) with masses of ~ 50 kDa were isolated from both subunits of RvH and isoform of Sepia officinalis, while seven FUs were purified from OvH. Further characterization of proteins by ESI-mass spectrometry (MS) and MALDI-MS, methods gave insights into post-translational modifications such as glycosylation. Glycosylation of O. vulgaris and S. officinalis Hcs was suggested based on the differences (11.6 and 40.0 kDa, respectively) between the masses measured by ESI-MS and those calculated by their gene sequences.
机译:对大分子复合物功能的理解主要与对其结构的精确了解有关。最近,合适的质谱技术(电喷雾电离(ESI)和基质辅助激光解吸/电离(MALDI))和多角度激光散射的发展已实现了对天然配合物及其亚基的质量测定。通过这些技术,已表征了软体动物章鱼,厚皮乌贼和Rapana venosa的大分子的结构和缔合/解离行为。头足类Hcs O.vulgaris(分别为3545和359.3 kDa)和Officinalis(分别为4134和443.8 kDa)的天然分子和解离分子的分子质量显示,只有一种类型的亚基可以组织其分子,而存在两种同工型。对于腹足动物R. venosa Hc,已经确定了具有不同质量(422.8和400.0 kDa)的物质,这些物质被聚集到双癸酰胺中。在用TPCK-胰蛋白酶进行有限的蛋白水解后,还确定了它们的结构亚基的差异。从RvH的两个亚基和棕褐色的亚型中分离出了质量约为50 kDa的八个功能单元,而从OvH中纯化了七个FU。通过ESI-质谱(MS)和MALDI-MS对蛋白质进行进一步表征,这些方法为翻译后修饰(例如糖基化)提供了见识。根据ESI-MS测定的质量与基因序列计算得到的质量之间的差异(分别为11.6和40.0 kDa),提出了普通麦草和厚皮草Hcs的糖基化作用。

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