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Lectin binding studies on murine peritoneal cells: Physicochemical characterization of the binding of lectins from Datura stramonium, Evonymus europaea, and Griffonia simplicifolia to murine peritoneal cells

机译:凝集素对鼠腹膜细胞的结合研究:延长素酸盐,evonymus的铕和Griffinia Simplicifolia与鼠腹膜细胞的凝集素结合的物理化学特征

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摘要

Purified 125I-labeled lectins from Datura stramonium, Evonymus europaea, and Griffonia simplicifolia (I-B4 isolectin) were used to analyze changes in the expression of carbohydrates on the surface of resident (PC) and thioglycollate-stimulated murine (C57B/6J) peritoneal exudate cells (PEC). The lectins from D. stramonium, E. europaea, and G. simplicifolia I-B4 bind specifically to PEC with relatively high affinity (Kd = 5.65 +/- 1.08 x 10-7 m, 1.08 +/- 0.12 x 10-8 m, and 1.33 +/- 0.15 x 10-7 m, respectively). Assuming a single lectin molecule binds to each cell surface saccharide, the number of receptor sites per cell ranged for different cell samples from 22.3 to 50.0 x 106, from 3.8 to 4.8 x 106, and from 2.0 to 16.8 x 106 for D. stramonium, E. europaea, and G. simplicifolia I-B4 lectins, respectively. There were approximately 3- to 7-fold, 16- to 20-fold, and 2-to 20-fold increases in binding capacity for D. stramonium, E. europaea and G. simplicifolia I-B4, respectively, compared to the binding to resident, peritoneal cells. Scatchard plots of the binding of all three lectins to PEC were linear, suggesting that the receptor sites for these lectins are homogeneous and noninteracting. The binding capacity of these lectins to PEC was unchanged after trypsin digestion of cells. The expression of carbohydrates on the surface of PEC was also monitored by an agglutination assay. PEC were agglutinated by all three lectins whereas PC either were not agglutinated or were agglutinated only at high lectin concentrations. On the basis of our knowledge of the carbohydrate binding specificity of the D. stramonium and G. simplicifolia I-B4 lectins, we postulate that, parallel with thioglycolate stimulation, there is an increase in the number of N-acetyllactosamine residues and terminal [alpha]--galactosyl end groups. The blood group B, and H type 1 determinants--Ga1[alpha]1,3[Fuc[alpha]1,2]Ga1[beta]1,3(or 4)GlcNAc and Fuc[alpha]1,2Ga1[beta]1,3G1cNAc, respectively, as well as Ga1[alpha]1,3Ga1[beta]1,3(or 4)GlcNAc--may be considered to be possible receptors for the E. europaea lectin. These glycoconjugates, present on the surface of peritoneal exudate cells, provide new chemical markers for studying the differentiation of resident peritoneal cells.
机译:纯化的125I型标记的凝胶素来自DaTura stramonium,evonymuseuropaea和Griffinia Silvericifolia(I-B4 isolectin)用于分析居民(PC)表面和硫糖苷刺激的鼠(C57b / 6j)腹膜表面上的碳水化合物表达的变化渗出物细胞(PEC)。来自D. stramonium,E.furopaea和G. Simpleicifolia I-B4的凝集素特异性与相对高亲和力的PEC(Kd = 5.65 +/- 1.08 x 10-7 m,1.08 +/- 0.12 x 10-8 m ,分别为1.33 +/- 0.15 x 10-7 m)。假设单章分子与每个细胞表面糖合结合,每个细胞的受体位点的数量为不同的细胞样品,从22.3-50.0×10 6,从3.8-4.8×10 6和2.0-16.8×106为D. stramonium, E. europaea和G. Simpleicifolia I-B4凝集素。与结合相比,D.Stamonium,E.Foulaea和G. SimpleCifolia I-B4的结合能力,约为3-至7倍,16至20倍和2-20倍的增加。居住,腹膜细胞。所有三章凝集素的螺旋曲线曲线曲线曲线是线性的,表明这些凝集素的受体位点是均匀的和非交互态的。在细胞的胰蛋白酶消化后,这些凝集素对PEC的结合能力不变。还通过凝集测定监测PEC表面上的碳水化合物的表达。 PEC由所有三章凝集凝集,而PC要么未凝集或仅在高凝集素浓度下凝集。在我们对D. Scramonium和G.的碳水化合物结合特异性的知识的基础上,我们假设,与硫代糖酸酯刺激平行,N-乙酰丙基胺残基和末端α的数量增加] - 半乳糖基端组。血液组B和H型测定剂 - GA1α1,3[FUCα1,2]Ga1β1,3(或4)GlcNAc和FUCα1,2GA1β1[β1] ]分别为1,3g1CNAC,以及Ga1α1,3ga1β1,3(或4)Glcnac - 可以被认为是E. europaea凝集素的可能受体。这些糖缀合在腹膜渗出物细胞表面上,为研究居民腹膜细胞的分化提供了新的化学标志物。

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