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Enzyme
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Query: EC:2.7.1.21 (
thymidine kinase
)
7,561
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
Using nuclear run-on assays, we showed that the tissue-specific expression of quail
Pax
-6 (
Pax
-QNR) P0-initiated mRNAs is due in part to regulation of the gene at the transcriptional level. Regulatory sequences governing neuroretina-specific expression of the P0-initiated mRNAs were investigated. By using reporter-based expression assays, we characterized a region within the
Pax
-QNR gene, located 7.5 kbp downstream from the P0 promoter, that functions as an enhancer in neuroretina cells but not in nonexpressing P0-initiated mRNA cells (quail embryo cells and quail retinal pigment epithelial cells). This enhancer element functioned in a position- and orientation-independent manner both on the
Pax
-QNR P0 promoter and the heterologous
thymidine kinase
promoter. Moreover, this enhancer element exhibited a developmental stage-specific activity during embryonic neuroretina development: in contrast to activity at day E7, the enhancer activity was very weak at day E5. This paralleled the level of expression of P0-initiated mRNAs observed at the same stages. Using footprinting, gel retardation, and Southwestern (DNA-protein) analysis, we demonstrated the existence of four neuroretina-specific nuclear protein-binding sites, involving multiple unknown factors. In addition we showed that the quail enhancer element is structurally and functionally conserved in mice. All of these results strongly suggest that this enhancer element may contribute to the neuroretina-specific transcriptional regulation of the
Pax
-6 gene in vivo.
...
PMID:Identification and characterization of a neuroretina-specific enhancer element in the quail Pax-6 (Pax-QNR) gene. 752 75
The murine paired box containing gene
Pax
-2 has been proposed to be involved in kidney and central nervous system (CNS) development. In this report, we show that expression cloning of
Pax
-2 cDNA allowed in vitro identification of specifically bound DNA sequences. When fused to the
thymidine kinase
(TK) promoter in front of reporter genes, these target sequences were able to mediate trans-activation by
Pax
-2 protein, thus demonstrating their in vivo function. Expression studies from adult mouse tissues revealed high levels of
Pax
-2 transcripts in male and female genital tracts, suggesting a second phase of
Pax
-2 activity. Sequence-specific DNA binding and subsequent modulation of promoter activities may constitute the molecular mechanism of
Pax
-2 action in specific adult tissues and during development.
...
PMID:Murine Pax-2 protein is a sequence-specific trans-activator with expression in the genital system. 851 25
We have identified alternatively spliced isoforms of murine Pax-3 and
Pax
-7 which differ by the presence or absence of a single glutamine residue in a linker region which separates two distinct DNA-binding subdomains within the paired domain. By reverse transcription-PCR, these isoforms of Pax-3 and
Pax
-7 (Q+ and Q-) were detected at similar levels through multiple developmental stages in the early mouse embryo. DNA-binding studies using the Q+ and Q- isoforms of Pax-3 revealed that this alternative splicing event had no major effect on the ability of these isoforms to bind to an oligonucleotide specific for the Pax-3 homeodomain (P2) or to a paired domain recognition sequence (e5) that interacts primarily with the N-terminal subdomain of the paired domain. However, DNA-binding studies with sequences (P6CON and CD19-2/A) containing consensus elements for both the N-terminal and C-terminal subdomains revealed that the Q- isoform binds to these sequences with a two- to fivefold-higher affinity; further mutation of the GTCAC core N-terminal subdomain recognition motif of CD19-2/A generated binding sites with a high degree of specificity for the Q- isoform. These differences in DNA binding in vitro were also reflected in the enhanced ability of the Q- isoform to stimulate transcription of a reporter containing multiple copies of CD19-2/A upstream of the
thymidine kinase
basal promoter. In support of the observations made with these naturally occurring Pax-3 isoforms, introducing a glutamine residue at the analogous position in PAX6 caused a fivefold reduction in binding to P6CON and a complete loss of binding to CD19-2/A and to the C-terminal subdomain-specific probe 5aCON. These studies therefore provide direct evidence for a role for the paired-domain linker region in DNA target site selection, and they identify novel isoforms of Pax-3 and
Pax
-7 that have the potential to mediate distinct functions in the developing embryo.
...
PMID:An alternative splicing event in the Pax-3 paired domain identifies the linker region as a key determinant of paired domain DNA-binding activity. 894 22
