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首页> 外文期刊>Journal of cell biology >Dynamics of toxin and lectin receptors on a lymphoma cell line and its toxin-resistant variant using ferritin-conjugated, 125I-labeled ligand.
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Dynamics of toxin and lectin receptors on a lymphoma cell line and its toxin-resistant variant using ferritin-conjugated, 125I-labeled ligand.

机译:使用铁蛋白缀合的125I标记的配体,淋巴瘤细胞系及其毒素抗性变异体上毒素和凝集素受体的动力学变化。

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The dynamics of the toxin Ricinus communis agglutinin II (RCAII or ricin) on cells of a murine lymphoma line (BW5147) and a toxin-resistant variant line (BW5147RicR.3) that is 200 times more resistant than the parent to direct RCAII cytotoxicity were examined using ferritin-conjugated, affinity purified, 125I-labeled RCAII (ferritin-125I-RCAII). Ferritin-125I-RCAII was indistinguishable from native RCAII in quantitative binding and cytotoxicity experiments. When RCAII-sensitive BW5147 and -resistant BW5147RicR.3 cells were labeled with ferritin-125I-RCAII at various toxin concentrations (1--10 microgram/ml), no differences in toxin binding were observed. These same cells were examined by electron microscopy. At low ferritin-125I-RCAII concentrations (1-3 microgram/ml RCAII) where only the parental BW5147 cells were significantly more sensitive to RCAII, toxin receptors were internalized by ferritin-125I-RCAII-induced endocytosis. In parallel experiments, ferritin-125I-RCAII that bound to the resistant BW5147RicR.3 cells remained relatively dispersed or clustered, and there was little evidence of transport into cells via endocytosis. At higher ferritin-125I-RCAII concentrations (greater than 7 microgram/ml RCAII) where both parental and resistant variant cells are sensitive to the cytotoxic effects of RCAII, more ferritin-conjugated toxin was bound, and subsequent endocytosis occurred to a similar degree in both cell types. Endocytosis of ferritin-conjugated concanavalin A was indistinguishable on RCAII-sensitive parental and resistant variant cells at all concentrations tested. The results suggest that a specific defect on the selected BW5147RicR.3 cells prevents RCAII entry into these cells a low toxin concentrations, rendering them more resistant to the cytotoxic effects of RCAII.
机译:鼠淋巴瘤细胞系(BW5147)和抗毒素变异株(BW5147RicR.3)的细胞上的毒素Ricinus communis凝集素II(RCAII或蓖麻毒蛋白)的动态性是其亲本对RCAII细胞毒性的200倍以上使用铁蛋白缀合,亲和纯化的125I标记的RCAII(铁蛋白125I-RCAII)进行检测。在定量结合和细胞毒性实验中,铁蛋白125I-RCAII与天然RCAII没有区别。当用各种毒素浓度(1--10微克/毫升)的铁蛋白-125I-RCAII标记RCAII敏感的BW5147和耐药的BW5147RicR.3细胞时,未观察到毒素结合的差异。通过电子显微镜检查这些相同的细胞。在低铁蛋白125I-RCAII浓度(1-3微克/毫升RCAII)下,只有亲本BW5147细胞对RCAII更加敏感,毒素受体被铁蛋白125I-RCAII诱导的内吞作用所内化。在平行实验中,与抗性BW5147RicR.3细胞结合的铁蛋白125I-RCAII保持相对分散或成簇,几乎没有证据显示通过内吞作用转运进入细胞。在较高的铁蛋白125I-RCAII浓度(大于7微克/ ml RCAII)下,亲本和耐药性变体细胞均对RCAII的细胞毒性作用敏感,结合了更多的铁蛋白结合毒素,随后的内吞作用发生在两种细胞类型。在所有测试浓度下,RCAII敏感的亲代和耐药变体细胞都无法区分铁蛋白缀合的伴刀豆球蛋白A的内吞作用。结果表明,所选BW5147RicR.3细胞上的特定缺陷可防止RCAII以低浓度的毒素进入这些细胞,从而使其对RCAII的细胞毒性作用更具抵抗力。

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