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2
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本文引用的文献

1
Phosphorylation of acetylhexosamines.N-乙酰己糖胺的磷酸化作用。
Arch Biochem Biophys. 1958 Mar;74(1):84-91. doi: 10.1016/0003-9861(58)90201-7.
2
Cystine transport is defective in isolated leukocyte lysosomes from patients with cystinosis.胱氨酸病患者分离出的白细胞溶酶体中胱氨酸转运存在缺陷。
Science. 1982 Sep 24;217(4566):1263-5. doi: 10.1126/science.7112129.
3
Defective cystine exodus from isolated lysosome-rich fractions of cystinotic leucocytes.胱氨酸病白细胞中富含溶酶体的分离组分的胱氨酸外排缺陷。
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4
ATP stimulates amino acid accumulation by lysosomes incubated with amino acid methyl esters. Evidence for a lysosomal proton pump.ATP刺激与氨基酸甲酯一起孵育的溶酶体积累氨基酸。溶酶体质子泵的证据。
J Biol Chem. 1981 Jun 25;256(12):6047-53.
5
Alterations in cultured fibroblasts of sibs with an infantile form of a free (unbound) sialic acid storage disorder.患有婴儿型游离(未结合)唾液酸贮积症的同胞培养成纤维细胞的改变。
Pediatr Res. 1983 May;17(5):307-12. doi: 10.1203/00006450-198305000-00001.
6
Patterns of amino acid efflux from isolated normal and cystinotic human leucocyte lysosomes.从分离出的正常和胱氨酸病患者的人白细胞溶酶体中氨基酸流出的模式。
J Biol Chem. 1982 Jun 10;257(11):6041-9.
7
N-acetylneuraminic acid and sialoglycoconjugate metabolism in fibroblasts from a patient with generalized N-acetylneuraminic acid storage disease.一名患有全身性N-乙酰神经氨酸贮积病患者成纤维细胞中N-乙酰神经氨酸和唾液酸糖缀合物的代谢
Biochim Biophys Acta. 1983 Oct 4;760(1):42-52. doi: 10.1016/0304-4165(83)90122-8.
8
Degradation of mucopolysaccharide in intact isolated lysosomes.完整分离的溶酶体中黏多糖的降解
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9
Sugar transport in rat liver lysosomes. Direct demonstration by using labelled sugars.大鼠肝脏溶酶体中的糖转运。使用标记糖的直接证明。
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10
Proteoglycans synthesized by smooth muscle cells derived from monkey (Macaca nemestrina) aorta.由源自猴(食蟹猴)主动脉的平滑肌细胞合成的蛋白聚糖。
J Biol Chem. 1983 May 10;258(9):5679-88.

糖蛋白和糖胺聚糖的溶酶体降解。硫酸盐和N - 乙酰己糖胺的外排与再循环。

Lysosomal degradation of glycoproteins and glycosaminoglycans. Efflux and recycling of sulphate and N-acetylhexosamines.

作者信息

Rome L H, Hill D F

出版信息

Biochem J. 1986 May 1;235(3):707-13. doi: 10.1042/bj2350707.

DOI:10.1042/bj2350707
PMID:3753439
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1146745/
Abstract

Lysosomal degradation of the carbohydrate portion of glycoproteins and glycosaminoglycans produces monosaccharides and sulphate, which must efflux from the lysosomes before re-entering biosynthetic pathways. We examined the degradation of glycoproteins and glycosaminoglycans by lysosomes isolated from cultured human diploid fibroblasts. Cells were grown for 24 h in medium containing [3H]glucosamine and [35S]sulphate. When lysosomes are isolated from these cells, they contain label primarily in macromolecules (glycoproteins and glycosaminoglycans). Glycoprotein degradation by isolated lysosomes was followed by measuring the release of tritiated sugars from macromolecules and efflux of these sugars from the organelles. Glycosaminoglycan degradation was monitored by the release of both tritiated sugars and [35S]sulphate. During macromolecule degradation, the total amounts of free [35S]sulphate, N-acetyl[3H]glucosamine and N-acetyl[3H]galactosamine found outside the lysosome parallels the amounts of these products released by degradation. The total degradation of glycoproteins and glycosaminoglycans by intact cultured cells was also examined. The lysosomal contribution to degradation was assessed by measuring inhibition by the lysosomotropic amine NH4Cl. After 48 h incubation, inhibition by NH4Cl exceeded 55% of glycoprotein and 72% of glycosaminoglycan degradation. Recycling of [3H]hexosamines and [35S]sulphate by intact cells was estimated by measuring the appearance of 'newly synthesized' radioactively labelled macromolecules in the medium. Sulphate does not appear to be appreciably recycled. N-Acetylglucosamine and N-acetylgalactosamine, on the other hand, are reutilized to a significant extent.

摘要

糖蛋白和糖胺聚糖碳水化合物部分的溶酶体降解产生单糖和硫酸盐,这些物质在重新进入生物合成途径之前必须从溶酶体中流出。我们研究了从培养的人二倍体成纤维细胞中分离出的溶酶体对糖蛋白和糖胺聚糖的降解作用。细胞在含有[3H]葡糖胺和[35S]硫酸盐的培养基中培养24小时。当从这些细胞中分离出溶酶体时,它们主要在大分子(糖蛋白和糖胺聚糖)中含有标记物。通过测量大分子中氚化糖的释放以及这些糖从细胞器中的流出,跟踪分离出的溶酶体对糖蛋白的降解。通过氚化糖和[35S]硫酸盐的释放来监测糖胺聚糖的降解。在大分子降解过程中,溶酶体外发现的游离[35S]硫酸盐、N-乙酰[3H]葡糖胺和N-乙酰[3H]半乳糖胺的总量与降解释放的这些产物的量平行。还研究了完整培养细胞对糖蛋白和糖胺聚糖的总降解。通过测量溶酶体促渗胺NH4Cl的抑制作用来评估溶酶体对降解的贡献。孵育48小时后,NH4Cl的抑制作用超过糖蛋白降解的55%和糖胺聚糖降解的72%。通过测量培养基中“新合成”的放射性标记大分子的出现来估计完整细胞对[3H]己糖胺和[35S]硫酸盐的再循环。硫酸盐似乎没有明显的再循环。另一方面,N-乙酰葡糖胺和N-乙酰半乳糖胺被大量再利用。