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N-糖基化不会影响蓖麻毒素 A 链的催化活性,但通过促进其从内质网输出而刺激细胞毒性。

N-glycosylation does not affect the catalytic activity of ricin a chain but stimulates cytotoxicity by promoting its transport out of the endoplasmic reticulum.

机构信息

Department of Plant Biology and Pathology, School of Environmental and Biological Sciences, Rutgers University, 59 Dudley Road, New Brunswick, NJ 08901-8520, USA.

出版信息

Traffic. 2012 Nov;13(11):1508-21. doi: 10.1111/j.1600-0854.2012.01404.x. Epub 2012 Sep 7.

Abstract

Ricin A chain (RTA) depurinates the α-sarcin/ricin loop after it undergoes retrograde trafficking to the cytosol. The structural features of RTA involved in intracellular transport are not known. To explore this, we fused enhanced green fluorescent protein (EGFP) to precursor (preRTA-EGFP), containing a 35-residue leader, and mature RTA (matRTA-EGFP). Both were enzymatically active and toxic in Saccharomyces cerevisiae. PreRTA-EGFP was localized in the endoplasmic reticulum (ER) initially and was subsequently transported to the vacuole, whereas matRTA-EGFP remained in the cytosol, indicating that ER localization is a prerequisite for vacuole transport. When the two glycosylation sites in RTA were mutated, the mature form was fully active and toxic, suggesting that the mutations do not affect catalytic activity. However, nonglycosylated preRTA-EGFP had reduced toxicity, depurination and delayed vacuole transport, indicating that N-glycosylation affects transport of RTA out of the ER. Point mutations in the C-terminal hydrophobic region restricted RTA to the ER and eliminated toxicity and depurination, indicating that this sequence is critical for ER exit. These results demonstrate that N-glycosylation and the C-terminal hydrophobic region stimulate the toxicity of RTA by promoting ER export. The timing of depurination coincided with the timing of vacuole transport, suggesting that RTA may enter the cytosol during vacuole transport.

摘要

蓖麻毒素 A 链(RTA)在逆行转运到细胞质后脱嘌呤α-菌毒素/蓖麻毒素环。RTA 参与细胞内运输的结构特征尚不清楚。为了探索这一点,我们将增强型绿色荧光蛋白(EGFP)融合到前体(preRTA-EGFP)中,其中包含 35 个残基的前导序列和成熟的 RTA(matRTA-EGFP)。两者在酿酒酵母中均具有酶活性和毒性。preRTA-EGFP 最初定位于内质网(ER),随后被转运到液泡,而 matRTA-EGFP 则留在细胞质中,表明 ER 定位是液泡转运的前提。当 RTA 中的两个糖基化位点发生突变时,成熟形式仍然具有完全的活性和毒性,表明这些突变不影响催化活性。然而,未经糖基化的 preRTA-EGFP 的毒性、脱嘌呤和延迟液泡转运能力降低,表明 N-糖基化影响 RTA 从 ER 中的转运。C 末端疏水区中的点突变将 RTA 限制在 ER 中,并消除了毒性和脱嘌呤作用,表明该序列对 ER 出芽至关重要。这些结果表明,N-糖基化和 C 末端疏水区通过促进 ER 输出来刺激 RTA 的毒性。脱嘌呤的时间与液泡转运的时间相吻合,表明 RTA 可能在液泡转运过程中进入细胞质。

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