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在聚丙烯酰胺和聚苯乙烯树脂载体上合成的肌红蛋白相关肽的抗原性。

The antigenicity of myoglobin-related peptides synthesised on polyacrylamide and polystyrene resin supports.

作者信息

Shi P T, Riehm J P, Todd P E, Leach S J

出版信息

Mol Immunol. 1984 Jun;21(6):489-96. doi: 10.1016/0161-5890(84)90064-6.

Abstract

Polyacrylamide resins [Atherton et al., Bioorg. Chem. 8, 351-370 (1979)] have been found suitable for solid-phase radioimmunoassay of peptides synthesised on the same supports; they are sufficiently stable during side-chain deprotection and swell sufficiently in aq. media to admit antibody molecules to the sites of peptide attachment. A re-examination of five synthetic peptide sequences corresponding to (15-21), (56-62), (94-99), (113-119) and (145-151) of beef myoglobin analogous to those delineated by Atassi [Immunochemistry 12, 423-438 (1975)] for sperm whale myoglobin shows that they all bind anti-beef myoglobin antibodies raised in rabbits, with binding capacities in the order V = III greater than IV greater than I = II. The resin-bound peptide (72-88) binds such antibodies even more extensively, as do certain sequential variants of peptide V. Other peptides, bound to polyacrylamide or polystyrene resins but unrelated to any of the five sequences and varying in size and amino acid composition and sequence were also tested with various antisera. It was concluded that the antibody binding properties of the 30 or so small peptides (two-seven residues) are dominated by their cationic and/or hydrophobic properties. In small peptides, therefore, antibody binding can be safely interpreted only in terms of general structural properties but not in terms of biological specificity. The latter property becomes assessable only with peptides representing larger areas of antigenic protein surfaces.

摘要

聚丙烯酰胺树脂[Atherton等人,《生物有机化学》8,351 - 370(1979)]已被发现适用于对在相同载体上合成的肽进行固相放射免疫分析;它们在侧链脱保护过程中足够稳定,并且在水性介质中充分溶胀,以使抗体分子能够进入肽附着位点。对与牛肉肌红蛋白的(15 - 21)、(56 - 62)、(94 - 99)、(113 - 119)和(145 - 151)相对应的五个合成肽序列进行重新研究,这些序列类似于Atassi[《免疫化学》12,423 - 438(1975)]为抹香鲸肌红蛋白所描述的序列,结果表明它们都能结合在兔体内产生的抗牛肉肌红蛋白抗体,结合能力顺序为V = III大于IV大于I = II。树脂结合的肽(72 - 88)结合此类抗体的程度甚至更高,肽V的某些连续变体也是如此。还使用各种抗血清测试了与聚丙烯酰胺或聚苯乙烯树脂结合但与五个序列中的任何一个无关且大小、氨基酸组成和序列各异的其他肽。得出的结论是,大约30个小肽(2 - 7个残基)的抗体结合特性主要由其阳离子和/或疏水特性决定。因此,对于小肽,仅根据一般结构特性而非生物学特异性来安全地解释抗体结合。只有对于代表抗原蛋白表面较大区域的肽,才能评估后者的特性。

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