“…Plasmids containing N-tubulin (Richter et al, 1988), Xenopus Krox-20 (Bradley et al, 1993), Xenopus Ap-2 (Winning et al, 1991), Xenopus Slug (Mayor et al, 1995), Xenopus Zic3 (Nakata et al, 1997), and Xenopus type I keratin (Miyatani et al, 1986) were linearized with restriction enzymes (StuI for N-tubulin, EcoRI for XKrox-20, HindIII for Xap-2, EcoRI for XSlug, BamHI for XZic3, and EcoRI for Xkeratin), and digoxygenin-labeled riboprobes were synthesized using T3 (for N-tubulinand XZic3) or T7 (for XKrox-20, Xap-2, and XSlug) or SP6 (for Xkeratin) polymerase. Wholemount in situ hybridization was essentially done as described by Harland (1991).…”