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. 1999 Oct;181(20):6403–6410. doi: 10.1128/jb.181.20.6403-6410.1999

TABLE 2.

Product yields from assays of dialyzed cell extracts of m-xylene-grown Azoarcus sp. strain Ta

Substrate added
Product (nmol)b
Product labeling
Aromatic compound Fumarate Succinyl-CoA CoA ATP Nitrate 3-MeBS E-3-MePI 3-Methylbenzoate
m-Xylene-d6 (360 nmol, total) + + 200 NDc ND Deuterium labeled
m-Xylene-d6 (360 nmol, total) + + + 73 85 ND Deuterium labeled
m-Xylene-d6 (360 nmol, total) + + + + 67 49 ND Deuterium labeled
m-Xylene-d6 (360 nmol, total) + + + 130 ND ND Deuterium labeled
3-MeBS (150 nmol, total) + 110 ND ND
3-MeBS (150 nmol, total) + + 64 40 ND
a

Each anoxic assay mixture (total volume, 1 ml) contained DTT (1 mM) as a reductant and dialyzed cell extracts (ca. 3 mg of protein). Initial concentrations of other substrates added are given as follows: fumarate, 500 μM; succinyl-CoA, 300 μM; CoA, 300 μM; ATP, 2 mM; and nitrate, 2 mM. A total of 360 nmol of m-xylene is equivalent to a liquid concentration of 170 μM. Assay mixtures were incubated for 1 h. Reaction products were extracted, derivatized to methyl esters, and analyzed by GC/MS. 

b

3-MeBS and 3-methylbenzoate were identified by GC/MS by using authentic standards. E-3-MePI was tentatively identified based on mass spectral similarity to an authentic E-PI standard. Assays were conducted in duplicate. Product yields of duplicate assays were typically within 5 to 20% of each other. Product yields shown are averages of the duplicate assays and are representative of other experiments conducted. 

c

ND, not detected. The detection limits of E-3-MePI and 3-methylbenzoate were less than 1 nmol.