Wilson P D, Firestone R A, Lenard J
J Cell Biol. 1987 May;104(5):1223-9. doi: 10.1083/jcb.104.5.1223.
The sensitivity of cultured human and hamster fibroblast cells to killing by the lysosomotropic detergent N-dodecylimidazole (C12-Im) was investigated as a function of cellular levels of general lysosomal hydrolase activity, and specifically of cysteine cathepsin activity. Fibroblasts from patients with mucolipidosis II (I-cell disease) lack mannose-6-phosphate-containing proteins, and therefore possess only 10-15% of the normal level of most lysosomal hydrolases. I-cell fibroblasts are about one-half as sensitive to killing by C12-Im as are normal human fibroblasts. Overall lysosomal enzyme levels of CHO cells were experimentally manipulated in several ways without affecting cell viability: Growth in the presence of 10 mM ammonium chloride resulted in a gradual decrease in lysosomal enzyme content to 10-20% of control values within 3 d. Subsequent removal of ammonium chloride from the growth medium resulted in an increase in lysosomal enzymes, to approximately 125% of control values within 24 h. Treatment with 80 mM sucrose caused extensive vacuolization within 2 h; lysosomal enzyme levels remained at control levels for at least 6 h, but increased 15-fold after 24 h of treatment. Treatment with concanavalin A (50 micrograms/ml) also caused rapid (within 2 h) vacuolation with a sevenfold rise in lysosomal enzyme levels occurring only after 24 h. The sensitivity of these experimentally manipulated cells to killing by C12-Im always paralleled the measured intracellular lysosomal enzyme levels: lower levels were associated with decreased sensitivity while higher levels were associated with increased sensitivity, regardless of the degree of vacuolization of the cells. The cytotoxicity of the cysteine proteases (chiefly cathepsin L in our cells) was tested by inactivating them with the irreversible inhibitor E-64 (100 micrograms/ml). Cell viability, protein levels, and other lysosomal enzymes were unaffected, but cysteine cathepsin activity was reduced to less than 20% of control values. E-64-treated cells were almost completely resistant to C12-Im treatment, although lysosomal disruption appeared normal by fluorescent visualization of Lucifer Yellow CH-loaded cells. It is concluded that cysteine cathepsins are the major or sole cytotoxic agents released from lysosomes by C12-Im. These observations also confirm the previous conclusions that C12-Im kills cells as a consequence of lysosomal disruption.
研究了培养的人及仓鼠成纤维细胞对溶酶体促透性去污剂N - 十二烷基咪唑(C12 - Im)杀伤作用的敏感性,该敏感性是一般溶酶体水解酶活性水平尤其是半胱氨酸组织蛋白酶活性水平的函数。黏脂贮积症II型(I细胞病)患者的成纤维细胞缺乏含6 - 磷酸甘露糖的蛋白质,因此大多数溶酶体水解酶的水平仅为正常水平的10% - 15%。I细胞成纤维细胞对C12 - Im杀伤作用的敏感性约为正常人成纤维细胞的一半。通过几种方式对CHO细胞的总体溶酶体酶水平进行实验性调控而不影响细胞活力:在10 mM氯化铵存在下生长,3天内溶酶体酶含量逐渐降至对照值的10% - 20%。随后从生长培养基中去除氯化铵,24小时内溶酶体酶增加至对照值的约125%。用80 mM蔗糖处理2小时内导致广泛空泡化;溶酶体酶水平在至少6小时内保持在对照水平,但处理24小时后增加15倍。用伴刀豆球蛋白A(50微克/毫升)处理也导致迅速(2小时内)空泡化,溶酶体酶水平仅在24小时后升高7倍。这些经实验调控的细胞对C12 - Im杀伤作用的敏感性始终与所测细胞内溶酶体酶水平平行:水平较低与敏感性降低相关,而水平较高与敏感性增加相关,无论细胞空泡化程度如何。通过用不可逆抑制剂E - 64(100微克/毫升)使其失活来测试半胱氨酸蛋白酶(在我们的细胞中主要是组织蛋白酶L)的细胞毒性。细胞活力、蛋白质水平和其他溶酶体酶未受影响,但半胱氨酸组织蛋白酶活性降至对照值的20%以下。E - 64处理的细胞几乎完全抵抗C12 - Im处理,尽管通过对加载路西法黄CH的细胞进行荧光观察,溶酶体破坏似乎正常。结论是半胱氨酸组织蛋白酶是C12 - Im从溶酶体释放的主要或唯一细胞毒性剂。这些观察结果也证实了先前的结论,即C12 - Im由于溶酶体破坏而杀死细胞。
