Department of Genetics and Genomic Sciences, Mount Sinai School of Medicine, New York, New York 10029.
Department of Genetics and Genomic Sciences, Mount Sinai School of Medicine, New York, New York 10029; Department of Developmental and Cell Biology, Sackler School of Medicine, Tel Aviv University, Tel Aviv, Israel 69978.
J Biol Chem. 2011 Oct 14;286(41):35624-35633. doi: 10.1074/jbc.M111.260372. Epub 2011 Aug 16.
Autoproteolytic cleavage of the inactive acid ceramidase (AC) precursor into the active heterodimer exposes a free cysteine residue, leading us to study whether AC could be regulated by one or more members of the cystatin family. Co-expression of the full-length AC and cystatin SA (cysSA) cDNAs led to significant reduction of AC activity in the transfected cells. Expression of cysSA also inhibited endogenous AC activity in cells and increased ceramide. Conversely, cysSA siRNA expression led to elevated AC activity and reduction in ceramide. The effects of cysSA siRNA expression could be reversed by the addition of recombinant cysSA into the culture media. These results were consistent with detection of a physical interaction between AC and cysSA, assessed by co-immunoprecipitation and nickel-nitrilotriacetic acid affinity chromatography, and further supported by co-localization of the endogenous proteins using confocal microscopy. In vitro kinetic analysis of purified, recombinant AC and cysSA confirmed the transfection results and suggested a non-competitive type of inhibition with a K(i) in the low micromolar range. Processing of the AC precursor into the active form was not affected by cysSA expression, suggesting that it likely inhibits AC by allosteric interference. Computer modeling and expression studies identified several potential inhibitory domains in cysSA, including a small "AC-like" domain (identical to the AC cleavage site, TICT). Small peptides, synthesized with combinations of this and a "cystatin-like" domain (QXVXG), exhibited significant AC inhibition as well. Such peptide-based AC inhibitors could potentially be used to regulate AC activity in cancer cells that are known to overexpress this enzyme alone and in combination with conventional anti-cancer drugs.
无活性酸性神经酰胺酶 (AC) 前体的自身蛋白水解裂解将活性异二聚体暴露出来一个游离半胱氨酸残基,这促使我们研究 AC 是否可以被胱抑素家族的一个或多个成员调节。全长 AC 和胱抑素 SA (cysSA) cDNA 的共表达导致转染细胞中的 AC 活性显著降低。cysSA 的表达也抑制了细胞内源性 AC 活性并增加了神经酰胺。相反,cysSA siRNA 的表达导致 AC 活性升高和神经酰胺减少。cysSA siRNA 表达的影响可以通过向培养物中添加重组 cysSA 来逆转。这些结果与通过共免疫沉淀和镍-亚氨基三乙酸亲和层析评估的 AC 和 cysSA 之间的物理相互作用一致,并通过使用共聚焦显微镜检测内源性蛋白的共定位得到进一步支持。纯化的重组 AC 和 cysSA 的体外动力学分析证实了转染结果,并表明存在一种非竞争性抑制类型,K(i) 值在低微摩尔范围内。cysSA 表达并不影响 AC 前体加工成活性形式,这表明它可能通过别构干扰抑制 AC。计算机建模和表达研究确定了 cysSA 中的几个潜在抑制结构域,包括一个小的“AC 样”结构域(与 AC 切割位点 TICT 相同)。合成的具有这种结构域和“胱抑素样”结构域(QXVXG)组合的小肽也表现出明显的 AC 抑制作用。这种基于肽的 AC 抑制剂可能可用于调节已知单独过表达这种酶的癌细胞以及与常规抗癌药物联合使用的 AC 活性。