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Homeobox-containing genes, which are characterized by a highly conserved 183 bp sequence known as a homeobox, encode sequence-specific DNA binding transcription factors. They have been shown to be involved in the specification of positional identity, segmentation, and body pattern during Drosophila development (1). On the basis of their regulated temporal and spatial expression during embryogenesis, homeobox-containing genes of the 5' end of the Hoxd cluster (formerly named the Hox 4 cluster) (2), are thought to be involved in the regulation of pattern formation and specification of positional information during vertebrate limb development (3, 4, 5). In order to isolate cDNA clones corresponding to chicken Hoxd-13 (formerly called CHox-4.8 or CHox-4g) (2), we have screened a cDNA library prepared from RNA isolated from 4-6 days (Hamburger-Hamilton stage 22-30) (6) embryonic chick limb buds with a polymerase chain reaction generated probe. The probe was prepared by amplification of an aliquot of the same library using amplification primers (5'-primer, 5'-CGAGATGTGCGT- CTACC-3'; 3'-primer, 5' CTGTCCGCAAGGAATCG-3') designed from the available chicken genomic Hoxd-13 sequence (4). Ten positive clones were isolated and sequenced. The map of the Hoxd-13 mRNA derived from the cDNA clones is shown in figure Based on comparisons of the nucleotide and deduced amino acid sequences with the published genomic sequence for the 2nd exon of the chicken (4, 5, 7), mouse (7) and human (8) genes, the clones were confirmed to correspond to chicken Hoxd-13. The deduced amino sequence is identical to the published amino acid sequences for human (8) and mouse Hoxd-13 (7) homeodomains, but differs from the homeodomains of human HOXA13 and HOX C13 (the paralogs of Hoxd-13 in HoxA and C cluster) (9) by 9 amino acids. Two out often clones contain sequence at their 5' ends, which is different from the sequence in the other clones. Based on identity with the genomic clone (4, 7), the position of the intron in other Hox genes, and sequence with homology to the 3' splice acceptor consensus sequence, this sequence appears to correspond to a retained intron. Clones which appeared to be primed at 2 different polyadenylation sites were obtained. Four were primed at the 3' site, and 3 at the more 5' polyadenylation site. A probe 5' to the more proximal polyadenylation site hybridized to mRNAs of approximated 1.6 and 2.5 kb whereas a probe 3' to the proximal polyadenylation site hybridized only to the 2.5 kb RNA (figure B 2). Three clones appeared to be primed on internal A- rich regions.
Rogina et al. (Fri,) studied this question.