The acetylating enzyme, spermidine/spermine N 1 -acetyltransferase, participates in polyamine homeostasis by regulating polyamine export and catabolism. Previously, we reported that overexpression of the enzyme in cultured tumor cells and mice activates metabolic flux through the polyamine pathway and depletes the N 1 -acetyltransferase coenzyme and fatty acid precursor, acetyl-CoA. Here, we investigate this possibility in spermidine/spermine N 1 -acetyltransferase transgenic mice in which the enzyme is systemically overexpressed and in spermidine/spermine N 1 -acetyltransferase knock-out mice. Tissues of the former were characterized by increased N 1 -acetyltransferase activity, a marked elevation in tissue and urinary acetylated polyamines, a compensatory increase in polyamine biosynthetic enzyme activity, and an increase in metabolic flux through the polyamine pathway. These polyamine effects were accompanied by a decrease in white adipose acetyl-and malonyl-CoA pools, a major (20-fold) increase in glucose and palmitate oxidation, and a distinctly lean phenotype. In SSAT-ko mice, the opposite relationship between polyamine and fat metabolism was observed. In the absence of N 1 -acetylation of polyamines, there was a shift in urinary and tissue polyamines indicative of a decline in metabolic flux. This was accompanied by an increase in white adipose acetyl-and malonyl-CoA pools, a decrease in adipose palmitate and glucose oxidation, and an accumulation of body fat. The latter was further exaggerated under a high fat diet, where knock-out mice gained twice as much weight as wild-type mice. A model is proposed whereby the expression status of spermidine/spermine N 1 -acetyltransferase alters body fat accumulation by metabolically modulating tissue acetyl-and malonyl-CoA levels, thereby influencing fatty acid biosynthesis and oxidation.The polyamines putrescine (Put), 3 spermidine (Spd), and spermine (Spm) are known for their critical role in supporting cell proliferation, albeit in ways that have not yet been clearly defined. For the most part, polyamines do not incorporate into macromolecules but rather bind electrostatically to negatively charged molecules, such as DNA, RNA, and phospholipids. Thus, as metabolically distinct entities, homeostatic control of intracellular polyamines is critical to their role in supporting cell proliferation. This is achieved by effector systems that regulate biosynthesis, catabolism, uptake, and export of these molecules. The enzyme, spermidine/spermine N 1 -acetyltransferase (SSAT), catalyzes the transfer of acetyl groups from acetyl-CoA to the terminal amines of polyamines and, thus, readies the molecule for export or catabolism via polyamine oxidase. The enzyme is short lived, sensitively regulated by intracellular polyamine pools, and highly inducible by polyamine analogues and various cytotoxic agents (1, 2).Although most antiproliferative strategies targeting the polyamine pathway seek to deplete intracellular pools by inhibiting biosynthesis, we have been investigating t...
Expression of spermine/spermidine-N1-acetyltransferase (SSAT), the rate-limiting enzyme of polyamine backconversion cascade, increases after ischemia-reperfusion injuries (IRI). We hypothesized that SSAT plays an important role in the mediation of IRI. To test our hypothesis, wild-type (SSAT-wt) and SSAT-deficient (SSAT-ko) mice were subjected to liver or kidney IRI by ligation of hepatic or renal arteries. The liver and kidney content of putrescine (Put), a downstream by-product of SSAT activity, increased in SSAT-wt animals but not in SSAT-ko animals after IRI, indicating that polyamine backconversion is not functional in SSAT-deficient mice. When subjected to hepatic IRI, SSAT-ko mice were significantly protected against liver damage compared with SSAT-wt mice. Similarly, SSAT-ko animals subjected to renal IRI showed significantly greater protection against damage to kidney tubules than SSAT-wt mice. These studies indicate that SSAT-deficient animals are protected against IRI and suggest that SSAT is an important mediator of the tissue damage in IRI.
N 1 ,N 11 -diethylnorspermine (DENSPM) is a polyamine analog that down-regulates polyamine biosynthesis and potently upregulates the polyamine catabolic enzyme spermidine/spermine N 1 -acetyltransferase (SSAT). In certain cells, such as SK-MEL-28 human melanoma cells, induction of SSAT is associated with rapid apoptosis. In this study, we used small interfering RNA (siRNA) to examine the role of SSAT induction in mediating polyamine pool depletion and apoptosis. siRNA duplexes were designed to target three independent sites in the SSAT mRNA coding region (siSSAT). When transfected under nontoxic conditions, two of the duplexes selectively reduced basal SSAT mRNA in HEK-293 cells by Ͼ80% and prevented DENSPM-induced SSAT mRNA by 95% in SK-MEL-28 cells.Treatment of SK-MEL-28 cells with 10 M DENSPM in the presence of 83 nM siSSAT selectively prevented the 1400-fold induction of SSAT activity by ϳ90% and, in turn, prevented analog depletion of spermine (Spm) pools by ϳ35%. siSSAT also prevented DENSPM-induced cytochrome c release and caspase-3 cleavage at 36 h and apoptosis at 48 h as measured by annexin V staining. Overall, the data directly link analog induction of SSAT to Spm pool depletion and to caspasedependent apoptosis in DENSPM-treated SK-MEL-28 cells. This represents the first use of siRNA technology directed toward a polyamine gene and the first unequivocal demonstration that SSAT induction initiates events leading to polyamine analog-induced apoptosis.The cellular requirement for polyamines in cell growth is typically met in all cells by a complex system of intracellular polyamine pool maintenance that involves homeostatic balancing of biosynthesis, catabolism, uptake, and export of polyamines. Of these, polyamine catabolism and polyamine export are regulated by an acetylation reaction catalyzed by SSAT. The enzyme acetylates spermine (Spm) and spermidine (Spd) to form N
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