Iso-coenzyme A

Burns, Kristi L.; Gelbaum, Leslie T.; Sullards, M. Cameron; Bostwick, D. E.; May, Sheldon W.

doi:10.1074/jbc.m411898200

Cited by 21 publications

(21 citation statements)

References 59 publications

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“…The 2′-phosphate isomer of coenzyme A isomer is called isocoenzyme A [25]. Burns and coauthors [16] separated CoASH and iso-CoASH as well as several pairs of acylCoA and acyl-iso-CoA in commercially available standards via RPLC and characterized those using MS/MS and NMR. They discovered that iso-CoAs acted as substrates instead of CoAs in enzyme-catalyzed reactions.…”

Section: Resultsmentioning

confidence: 99%

“…Reversed phase liquid chromatography employing ion-pairing reagents (ion-pair RPLC) was addressed as the method of choice suitable for a broad spectrum of short-chain acyl-CoA analysis [11,12,13,14,15]. Alternately, a comparatively smaller selection of these target metabolites has been separated by reversed phase liquid chromatography without the use of ion-pairing reagents [16,17,18,19]. In studies where short-chain acyl-CoAs were measured within a comprehensive primary metabolome analysis, ion-pair RPLC was applied [20,21].…”

Section: Introductionmentioning

confidence: 99%

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LC-MS/MS-based analysis of coenzyme A and short-chain acyl-coenzyme A thioesters

et al. 2015

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Absolute quantification of intracellular coenzyme A (CoA), coenzyme A disulfide, and short-chain acyl-coenzyme A thioesters was addressed by developing a tailored metabolite profiling method based on liquid chromatography in combination with tandem mass spectrometric detection (LC-MS/MS). A reversed phase chromatographic separation was established which is capable of separating a broad spectrum of CoA, its corresponding derivatives, and their isomers despite the fact that no ion-pairing reagent was used (which was considered as a key advantage of the method). Excellent analytical figures of merit such as high sensitivity (LODs in the nM to sub-nM range) and high repeatability (routinely 4 %; N = 15) were obtained. Method validation comprised a study on standard purity, stability, and recoveries during sample preparation. Uniformly labeled U(13)C yeast cell extracts offered ideal internal standards for validation purposes and for a quantification exercise in the rumen bacterium Megasphaera elsdenii.

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Section: Resultsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

LC-MS/MS-based analysis of coenzyme A and short-chain acyl-coenzyme A thioesters

et al. 2015

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“…These data indicated that BrPA was directly interfering with CoA at its free thiol group. Using a previously published ionization pattern for CoA (29), we demonstrated by mass spectrometry that pyruvylation occurs at the sulfhydryl group of CoA (Supplementary Fig. S6).…”

Section: Brpa Inhibits Dnl By Pyruvylation Of Coamentioning

confidence: 99%

Metabolic Vulnerabilities in Endometrial Cancer

et al. 2014

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Women with metabolic disorders, including obesity and diabetes, have an increased risk of developing endometrial cancer. However, the metabolism of endometrial tumors themselves has been largely understudied. Comparing human endometrial tumors and cells with their nonmalignant counterparts, we found that upregulation of the glucose transporter GLUT6 was more closely associated with the cancer phenotype than other hallmark cancer genes, including hexokinase 2 and pyruvate kinase M2. Importantly, suppression of GLUT6 expression inhibited glycolysis and survival of endometrial cancer cells. Glycolysis and lipogenesis were also highly coupled with the cancer phenotype in patient samples and cells. To test whether targeting endometrial cancer metabolism could be exploited as a therapeutic strategy, we screened a panel of compounds known to target diverse metabolic pathways in endometrial cells. We identified that the glycolytic inhibitor, 3-bromopyruvate, is a powerful antagonist of lipogenesis through pyruvylation of CoA. We also provide evidence that 3-bromopyruvate promotes cell death via a necrotic mechanism that does not involve reactive oxygen species and that 3-bromopyruvate impaired the growth of endometrial cancer xenografts Cancer Res; 74(20); 5832-45. Ó2014 AACR.

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“…These species were absent in control samples and their MS/MS fragmentation pattern was consistent with that of coenzyme A derivatives. [43] While the assignment of m/z 922 (Figure 1 A) and 964 (Figure 1 B) to the diketide 21 a and the triketide 22 a, respectively, was clear-cut, two distinct peaks were found for m/z 1006 at 15.9 and 19.9 min (Figure 1 C and E). Their different MS/MS fragmentation patterns allowed their assignment to the nonhydrolyzable tetraketide 23 a (Figure 1 C) and to the dehydrated, possibly cyclized, natural tetraketide 25, respectively (Figure 1 E), with the latter showing the m/z 768 fragment diagnostic for a coenzyme A thioester.…”

Section: Trapping Polyketide Intermediates Of the Sts Reactionmentioning

confidence: 92%

Malonyl carba(dethia)‐ and Malonyl oxa(dethia)‐coenzyme A as Tools for Trapping Polyketide Intermediates

2009

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In order to study intermediates in polyketide biosynthesis two nonhydrolyzable malonyl coenzyme A analogues were synthesised by a chemoenzymatic route. In these analogues the sulfur atom of CoA was replaced either by a methylene group (carbadethia analogue) or by an oxygen atom (oxadethia analogue). These malonyl-CoA analogues were found to compete with the natural extender unit malonyl-CoA and to trap intermediates from stilbene synthase, a type III polyketide synthase (PKS). From the reaction of stilbene synthase with its natural phenylpropanoid substrates, diketide, triketide and tetraketide species were successfully off-loaded and characterised by LC-MS. Moreover, the reactivity of the nonhydrolyzable analogues offers insights into the flexibility of substrate alignment in the PKS active site for efficient malonyl decarboxylation and condensation.

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Iso-coenzyme A

Cited by 21 publications

References 59 publications

LC-MS/MS-based analysis of coenzyme A and short-chain acyl-coenzyme A thioesters

LC-MS/MS-based analysis of coenzyme A and short-chain acyl-coenzyme A thioesters

Metabolic Vulnerabilities in Endometrial Cancer

Malonyl carba(dethia)‐ and Malonyl oxa(dethia)‐coenzyme A as Tools for Trapping Polyketide Intermediates

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