. 1999 May;65(5):2143–2150. doi: 10.1128/aem.65.5.2143-2150.1999

TABLE 2.

Microbial cultures used to prepare reference DNAs for initial optimization of probe hybridization conditions and routine probe calibration

Taxonomic group and organism	Culture source^b
Eucarya
Penicillium crustosum^a	1
Archaea
Methanobacterium formicicum^a	2
Bacteria
Proteobacteria
α
Azospirillum brasilense^a	3
Rhodospirillum rubrum	4
Sinorhizobium meliloti	5
Rhizobium loti	5
β
Burkholderia cepacia	6
Alcaligenes sp.^a	7
γ
Escherichia coli^a	8
Pseudomonas fluorescens	9
Pseudomonas aureofaciens	9
Serratia plymuthica^a	9
Xanthomonas campestris	9
Enterobacter cloacae	9
Azotobacter vinelandii	4
Klebsiella pneumoniae	10
δ
Desulfovibrio desulfuricans^a	11
Gram positive
Low G+C
Bacillus cereus	9
High G+C
Arthrobacter oxydans	12
Arthrobacter globiformis^a	12
Streptomyces bikiniensis	12
Streptomyces coelicolor	12
Streptomyces griseus	12

DNA from this organism was used for routine probe calibration.

Sources were as follows: 1, J. Parke (University of Wisconsin-Madison); 2, P. Weimer (University of Wisconsin-Madison); 3, American Type Culture Collection (ATCC; Rockville, Md.) strain 29145; 4, G. Roberts (University of Wisconsin-Madison); 5, J. Lindquist (University of Wisconsin-Madison); 6, S. Fetzner (University of Hohenheim); 7, R. C. Wyndham (Carleton University); 8, authors’ lab collection; 9, R. Zablotowicz (U.S. Department of Agriculture-ARS, Stoneville, Miss.); 10, B. Thede (Ciba-Giegy Corp., Greensboro, N.C.); 11, ATCC strain 27774; and 12, J. Ensign (University of Wisconsin-Madison).