The fec locus encodes a citrate-mediated Fe3+ transport system. Six mutations in fec were mapped by conjugation experiments at min 7 (13) of the Escherichia coli linkage map (1), which supported the biochemical distinction (3) of the citrate iron transport system from the iron transport systems mediated by enterochelin (enterobactin) and the hydroxamate siderophores. Phage P1 cotransduction offec with markers in the 7-min region (lac and proAB) failed (5, 13). Cotransduction with argF was complicated by the occurrence of two genes, argF at min 7 and argI at min 97, both of which encode the same enzyme, ornithine carbamoyltransferase. The initial localization offec at min 7 could be due to erroneous conjugation experiments in which argI at min 97 instead of argF at min 7 was transferred.fec is composed of seven contiguous genes, of whichfecI and fecR regulate transcription of the fecABCDE transport genes (2, 7, 9, 11). Sequencing of the entire fec region (7, 9, 11) revealed an ISI element, upstream of the fecIRABCDE operon (11), which is 100% identical to the sequence of ISlF at min 97.5 (10). The other ISJ elements sequenced (listed in references 9 and 10), which include ISIB and ISIC at min 6.3 and 6.5, respectively, show only 85.5 to 85.6% sequence identity with ISI upstream of fecI. To clarify the conflicting data, we hybridized DNA probes isolated from fecR (BglI-PstI fragment), fecA (PstI-PvuI fragment), and fecB (PvuI-SalI fragment) with lambda phages of the Kohara "miniset" library carrying DNA fragments of the 7-and 97-min regions ofE. coli K-12 W3110 (6). All three fec probes hybridized to phage 7G7 (662), the fecR and fecA probes hybridized to phage 9H9 (663), and there was no hybridization to phage E4D8 (660) of the 97-min region or to phages 9G4 (134), 6E6 (135), 1F6 (136), 9F1 (137), and 10A6 (138) of the 7-min region. This result clearly demonstrates that thefec genes are located at min 97.3 of the E. coli K-12 chromosome and not at min 7 (Fig.
