. 2006 Sep;80(17):8422–8438. doi: 10.1128/JVI.02601-05

TABLE 2.

Primers used to prepare plasmids expressing EGFP-M2 truncations

Construct^a	Primer sequence (5′ to 3′)^b
Construct^a	Forward	Reverse
pEGFP-N-M2(1-41)	CGATTCCTCGAGGCAAAGATGGGGAACGC	CGATCGAAGCTTATTTAACATTCCAGGTG
pEGFP-C-M2(582-708)	ATACTCGAGGAATGGGTGTACGGATATTCAATC	AAGCTTTCAGCGTGTATACCCACGCTTAACC
pEGFP-C-M2(585-708)	ATCTCGAGGTATATTCAATCCCAAAGGAATTCTC	ATAAGCTTTCAGCGTGTATACCCACGCTTAACCAC
pEGFP-C-M2(610-675)	ATCTCGAGCAATTACGCAGGCAGCACCGGT	TATAAGCTTTCAAGGCGCTGGAAAGTGCGTCGA
pEGFP-C-M2(582-611)	ATACTCGAGGAATGGGTGTACGGATATTCAATC	TAAAGCTTTCAAATAATTGTACTTGGATCACC
pEGFP-N-M2(582-611)	ATACTCGAGGAATGGGTGTACGGATATTCAATC	TAAAGCTTAATAATTGTACTTGGATCACC
pEGFP-C-M2(582-643)	ATACTCGAGGAATGGGTGTACGGATATTCAATC	ATAAGCTTCACCCCGCCGATAAACTTTTAGTACG
pEGFP-C-M2(582-675)	ATACTCGAGGAATGGGTGTACGGATATTCAATC	TATAAGCTTTCAAGGCGCTGGAAAGTGCGTCGA
pEGFP-C-M2(582-675ΔH2)^c	(i) ACCCCAACGAGAAGCGCGATCAC	(ii) ACCCCCGCCGATAAACTTTTAGTAATAATTGTACTTGGATCACC
	(iii) TGATCCAAGTACAATTATTACTAAAAGTTTATCGGCGGGGGTG	(iv) TGGACAAACCACAACTAGAATGCAGTG

Each construct was designed to express an EGFP fusion including the indicated amino acid residues of μ1. The pEGFP-C1 and -N1 vectors and all PCR products were digested with XhoI and HindIII for cloning.

Forward primers are in the same orientation as the coding strand; reverse primers are in the reverse orientation to the coding strand. Restriction enzyme sites are in italics, and the inserted start and stop codons are underlined.

Primer pairs i and ii amplified a region in pEGFP-C-M2(582-675) from within EGFP to M2 residue 611. Additional sequence in reverse primer ii (bold type) was complementary to the 5′ sequence of M2(637-675). Primer pairs iii and iv amplified a region in pEGFP-C-M2(582-675) from M2 residue 637 to a region in the vector downstream of the M2 gene. Additional sequence in forward primer iii (bold type) was complementary to sequence at the 3′ end of M2(582-611).