2010
DOI: 10.1194/jlr.d010033
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A simple fluorogenic method for determination of acid ceramidase activity and diagnosis of Farber disease

Abstract: This article is available online at http://www.jlr.org hydrolase encoded by the ASAH1 gene. The main clinical features include painful and progressively deformed joints, subcutaneous nodules, a hoarse cry due to laryngeal involvement, and premature death. Hepatosplenomegaly and nervous system dysfunction may also occur ( 1, 2 ). Although the pathogenesis of FD is still unclear in terms of the molecular lesions caused by ceramide storage, the involvement of aCDase defi ciency is unquestionable. Recent interest … Show more

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Cited by 54 publications
(49 citation statements)
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“…In agreement with the AC activity of NAAA, in this article, we show that NAAA hydrolyzes acceptor FRET pairs are located as part of the acyl chain and/or the sphingoid base of the substrate, and fl uorescence is displayed by the ceramidase hydrolysis-promoted fl uorescence quencher release. On the other hand, a series of fl uorogenic coumarin-containing ceramidase substrates has also been described ( 10,11 ). These compounds (RBM14 compounds, Fig.…”
Section: Discussionmentioning
confidence: 99%
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“…In agreement with the AC activity of NAAA, in this article, we show that NAAA hydrolyzes acceptor FRET pairs are located as part of the acyl chain and/or the sphingoid base of the substrate, and fl uorescence is displayed by the ceramidase hydrolysis-promoted fl uorescence quencher release. On the other hand, a series of fl uorogenic coumarin-containing ceramidase substrates has also been described ( 10,11 ). These compounds (RBM14 compounds, Fig.…”
Section: Discussionmentioning
confidence: 99%
“…1 ), to determine AC activity. Other analogs of RBM14C16 with different N -acyl chain lengths were later reported as AC substrates and for use in diagnosis of Farber disease ( 11 ). Among the several analogs, RBM14C12 was the preferred substrate for AC.…”
Section: Knockdown Of Acer3 In Hct116 Cellsmentioning
confidence: 99%
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“…For the assay, 75 µl of reaction buffer (100 mM sodium acetate buffer, pH 4.5, for acid ceramidase activity), containing 40 µM RBM14C12 fl uorogenic substrate ( 22 ) (with or without test compounds), was mixed with 25 µl of the cell lysates (20 µg of total protein content) and incubated at 37°C for 3 h. For time dependence of inhibition, incubations were carried out for 0.5, 1, 2, and 3 h with different amounts of protein. The reaction was stopped by addition of methanol followed by NaIO 4 (2.5 mg/ml in 200 mM glycine/NaOH buffer, pH 10.6).…”
Section: Fluorogenic Ceramidase Assaymentioning
confidence: 99%