Table 2.

Oligonucleotide primers and PCR conditions used in this study

				Cycle
Primer name and amplified region	Primer sequence
Primer name and amplified region	Primer sequence	Cycles	Hot start	Denaturation	Annealing	Extension	Final extension
16S rRNA^**	IF 5′-AGA GTT TGA TCM TGG CTC AG-3′		94 °C	94 °C	49 °C	72 °C	72 °C
	4R 5′-AGG CCT TCT TCA TAC ACG CG-3′	25	2 min	15 s	15 s	15 s	7 min
16S rRNA^**	2F 5′-GCA AGC CTG ATG CAG CCA TG-3′		94 °C	94 °C	49 °C	72 °C	72 °C
	3R 5′-ATC GTT TAC GGC GTG GAC TA-3′	25	2 min	15 s	15 s	15 s	7 min
16S rRNA^**	3F 5′-AAA CAG GAT TAG ATA CCC TG-3′		94 °C	94 °C	49 °C	72 °C	72 °C
	2R 5′-CTG GTC GTA AGG GCC ATG AT-3′	25	2 min	15 s	15 s	15 s	7 min
16S rRNA^**	4F 5′-AGG TGG GGA TGA CGT CAA GT-3′		94 °C	94 °C	49 °C	72 °C	72 °C
	1R 5′-AAG GAG GTG WTC CAR CC-3′	25	2 min	15 s	15 s	15 s	7 min
luxA-specific^*	F 5′-GTTCTTAGTTGGATTATTGG-3’		94 °C	94 °C	44 °C	72 °C	72 °C
Positions 568–995	R 5′-TCAGTTCCCATTAGCTTCAAATCC-3’	29–33	2 min	15 s	30 s	30 s	7 min
1st luxA^†	F 5′-CAGAATCACCAAAAAGGAATAGGT-3’	30	94 °C	94 °C	55 °C	72 °C	72 °C
Positions 1–590	R 5′-CAATTTCATTATAGAGTTCCATCTGTG-3’		2 min	15 s	30 s	30 s	7 min
2nd luxA^†	F 5′-GTTCTTAGTTGGATTATTGGTA-3’	26–30	94 °C	94 °C	50 °C	72 °C	72 °C
Positions 450–1068	R 5′-AACTTGTTCCTTATTATCTCTAGTAT-3’		2 min	15 s	30 s	30 s	7 min
luxA 1–569^†	F 5′-GCGAAGATTAAGAAATAAAA-3’	25–30	94 °C	94 °C	47 °C	72 °C	72 °C
Positions 1–569	R 5′-TTCTTTAGAGTACTTTGTTGG-3’		2 min	15 s	30 s	30 s	7 min
luxA 400–1168^†	F 5′-ATTTAATTTTGGTGTTGTTA-3’	25–30	94 °C	94 °C	43 °C	72 °C	72 °C
Positions (400–1168)	R 5′-TTATTTTTGAGGTTCTTTTA-3’		2 min	15 s	30 s	30 s	7 min
luxA 401–1168⁶	F 5′-TTTAATTTTGGTGTTGTT-3’	25–30	94 °C	94 °C	43 °C	72 °C	72 °C
Positions 401–1168	R 5′-TTATTTTTGAGGTTCTTTT-3’		2 min	15 s	30 s	30 s	7 min
luxA ext^†	F 5′-AATTTATTTAGGTTCTTTTAAG-3’	28	94 °C	94 °C	42.5 °C	72 °C	72 °C
	R 5′-AAYATTTRTTTTTCGTATCA-3’		2 min	15 sec	30 s	30 s	7 min
luxA intl^†	F 5′-CTATAATCAACACGTCGATTS-3’	28	94 °C	94 °C	48.4 °C	72 °C	72 °C
	R 5′-CAATGGTWCTTAGTTGGATTAT-3’		2 min	15 s	30 s	30 s	7 min
luxA int2^†	F 5′-CCATYTGTGYTTTTTTYTCATT-3’	28	94 °C	94 °C	48.5 °C	72 °C	72 °C
	R 5′-KTTTGATACATATTGGACSTT-3’		2 min	15 s	30 sec	30 s	7 min
luxA int3^†	F 5′-TGATAATCRTAACCWCGAGT-3’	28	94 °C	94 °C	47.5 °C	72 °C	72 °C
	R 5′-AAGGTCGWTTTAATTTTGG-3’		2 min	15 s	30 s	30 s	7 min
Pleiogleiog A^‡	F 5′-GTTTAAGATCAACTGTCTAAAGGRCG-3’	25–30	94 °C	94 °C	56 °C	72 °C	72 °C
	R 5′-TCAGAACCATTCGCTTCAAATCCAAC-3’		2 min	15 s	30 s	30 s	7 min
Pleiogleiog AB^‡	F 5′-CGTCGCCGACTTGATTACAGTAACG-3’	25–30	94 °C	94 °C	60 °C	72 °C	72 °C
	R 5′-ATCCTTTTCTTGCTGCCCATTCAACC-3’		2 min	15 s	30 s	30 s	7 min
Pphosp A^‡	F 5′-CTTTTAGATCCAATGTCAAAAGGCCG-3’	25–30	94 °C	94 °C	58 °C	72 °C	72 °C
	R 5′-TCAGAGCCATTTGCTTCGAAACCAAG-3’		2 min	15 s	30 s	30 s	7 min
Pphosp AB^‡	F 5′-AAACGTCGTGTTGATTATAGCAACG-3’	25–30	94 °C	94 °C	55.4 °C	72 °C	72 °C
	R 5′-TCCAACGATATGTTAGTGGAAGC-3’		2 min	15 s	30 s	30 s	7 min
luxAl27^§	F 5′-GANCANCANTTNACNGAGTTTGG-3’	30	94 °C	94 °C	58 °C	72 °C	72 °C
	R 5′-ATTTCNTCTTCAGNNCCATTNGCTTCAAANCC-3’		5 min	30 s	30 s	90 s	7 min
luxAf Wimpee^¶	F 5′-CTACTGGATCAAATGTCAAAAGGA-3’	30	94 °C	94 °C	56 °C	72 °C	72 °C
	R 5′-TCAGAACCGTTTGCTTCAAAACC-3’		5 min	1.5 min	30s	2 min	7 min
gapA^**	F 5′-GTG TAC TTC GAG CGT TAT AC-3′	29	95 °C	95 °C	40 °C	70 °C	70 °C
	5′-GCC CAT TAC TCA CCC TTG TT-3′		5 min	15 s	15 s	1 min	7 min

Lee and Ruby, 1995.

^†

Oligonucleotide primers designed in this study.

^‡

Ast and Dunlap, 2004.

^§

Modified from Budsberg et al., 2003.

^¶

Wimpee et al., 1991.

^**

Nishiguchi and Nair, 2003.