FlyBase Clone Report: Dmel\RE12101

General Information

Symbol

Dmel\RE12101

Species

D. melanogaster

Name

RE12101

FlyBase ID

FBcl0211225

Feature type

cDNA_clone

Computed gene(s)

Dmel\WASp

Collection Status

DGC gold BDGP

Known Problems

none

FlyBase assessment

Library

RE_cDNA

RE cap-trapped cDNA library of D. melanogaster, iso-1 strain, embryo (0-22 hr).

Strain

Vector

Tissue Source

Stage

Tissue/Position (including subcellular localization)

Reference

embryonic stage

organism

Comment: 0-22 hr AEL

(Stapleton et al., 2002)

Sequence Data of the Insert

Full Length Sequence

Total bases

2,162

NCBI

AY070576

Full Length sequence dataSequence Downloader

ATCGCCTTTTTCGGTCGGTCACACTGGCAGCAATTGAATTGGAGTGAAAAAAAATAAATGAATAAACAAACTAGCATTGC
GTCCGGGAACAGACGAATAATCAACCGAGGAACACTCGTTTTCAACGCCATGCACTCGATGACGCGGACGCGCGCACAGT
AGAGCCTCCCGATAAGAGTCCCGGAATCCGCAAGGCCAGAGACTACACAGATTTTGTGGGAAACCAGCCCAGATCCCCAT
ATCCAGCACCAGACCCAGATCCAACGAAACCGGCCAGATGAGCAGCGGAATGAGGTCGCAGGACGGTCCACGGGCGAAGG
TCAATGCCGCCAGTACGCTGCTCACCCAGGAGGAGAATGAGGCCGTCTTCAAGCTGCTGGGCAAGAAGTGCCAGACACTC
AACACCGCCGTGGTGCAGATCTACAAGACGGAGGGCAGCGCCCATGCCCACTGGAAGAAGCGACACACCGGGGTGGTGTG
CTTCGTCAAGGATAGCGCCATCCGATCCTATTTCATGCGCGCCTACTGCCTGATCAAGAACGAGCTAATCTGGGAGCACG
AGATCTACGATGGCATGGAGGTGGTCAAGTCGCGACCCTTTCTGCTTACCTTCGAGGGCAGTGATGGTCATGTGGGACTA
AACTTCGTGTCCGAGGAGGAGTGCGACTCCTTCTTCCGCATTGTGGACGCCACCATAGAGACGCGTAACCGCAAACGACA
AGAGAAACGCAACCGGCAGAAAAGCCAACAGGCGCCCAATGCTCCATTGCCTCAGGTGCAGCGGGAGCCGGCCAGGCCAC
CACCCATGCAAGGTGGGTTGTCCTCCACGGACGGCGTTCAGCTGAGGAACAACAAGATCAACTCGGTGACACTGACGCCT
GCACCAGCGCCAGCGCAGTCGAAGAATTTCCTATCCAGTAGCTTTGGTCTGGGCAACAATGCGAAGGACAAGAAGCGCAA
GGTGACCAAGGCGGACATCAGCCGGCCGACAAACTTTGTACACCTCAGCCACGTGGGCTGGGATGCGCAGAAGGGATTTG
ATCTGGCGGGCAACGAGAACGACGAAGTGCTGAACGAGTTCTTCGTGAAGGCAGGTGTCTCGGAAGTGGAGCTAAAAGAT
CGGGACACCCGCGCCTTCATCTACGACTTCATACAGAGCAACAATGTCCTGGCTTCGGTGAAGCAATACAGTGTAGAATC
CCCTACGGAAACAGCGGCTCCCATGCCACCACCGGTGCCAACCCGTCATCCATCTAATGGCAACCAAAGAACTGCTCCTC
CGCTGCCGCCGGCAAGACAACCACCGCCCGCAGTTCCCGTTACTGTGCCGGGCGCCGCACGAGCTCCTCCACCACCTAAC
AGACCACCACCCATTAGCACCGCTCCACCACCGCCACCAGTCAGTGCGCCTGTTGTGGCGCCGCCACCTCCACCACCGCC
ACCACCAGCAGCGGTGCCGCCACCACCGCCCCCGCCCATGCCAGTGGGAGAGATCCCCGTCATTACGACCACGCACGCAC
CGACTCAAGCAGCCCGGCCAGCAGCTCCGGCGGCTCCAGATCCACGCAATGCACTGATGGACGCCATACGCAAGGGAACC
CAGCTGAAGAAAGTGGACACGACTGCTCTCAGCACTGGAAGTGGCGACTCACGCAGCGATTTAATGAAGGATATCCGTCA
GGGCACTGTTTTGAAGCCGGCCAAGGAACGGGAGCTGGGCAGTCAGCGAAACAGCGACAGTGGAGCAGGCACTGACGCAT
TGGCCGATGCACTGCGTCGAGCGCTGGCGGCGCGTGGAAACGCCATCCACTCGGATGAGGACGAAACCGAGTCCTCGGAC
AACGAAGGGGAGTGGGACTAAGGGAACTACGAATGACACGATGCGATAGGGGCAGGCAGACACTATTCCAAAAATAAGCA
ATAATTTAATTTGTGCTTTGGCATTTTGGTTTATCGTTAGATAAATCCCTGTAAATACTGTTAGTGAATTTTCATACCTC
TTTAATTTAATTGTACGCGCTTAACAAAAACAAAATCTACTAAAGGATAATCACAAATTGAGAAATTTTATCAGCAATTA
CCCGTTTTCGTTTGTTCCAAATCACATTTGCATATCCATAAAGCTGCTCAATTAAATATGAATAATAAAAAAAAAAAAAA
AA

Library Information (1)

Library: RE_cDNA

Description

Cloned cDNAs prepared from polyadenylated RNA isolated from 0-22-hr embryos.

(Stapleton et al., 2002)

Sample preparation

For the RE cDNA library, embryos at 0-22 hr AEL were collected from an isogenic y; cn bw sp (iso-1) strain.

Protocol

RNA was polyA+ selected twice (RNA made by L. Hong). cDNA was synthesized by priming with the oligo(dT) primer adapter (5'-GAGAGAGAGAGGATCCAATACTGGAGAGTTTTTTTTTTTTTTTTVN-3'). The first strand was synthesized in presence of trehalose, which increases the full-length cDNA synthesis (Carninci, P. et al. 1998. Proc. Natl. Acad. Sci. U.S.A. 95(2): 520-524; Carninci, P. et al. 1999. Methods Enzymol. 303: 19-44). Full-length cDNA was selected with the biotinylated cap-trapper (Carninci, P. et al. 1996. Genomics 37(3): 327-336). A linker was then ligated to the single-strand cDNA following the published protocol (Shibata, Y., et al. 2001. Biotechniques 30(6): 1250-1254). Subsequently, the cDNA was normalized by using RoT=1.0 as published (Carninci, P., et al. 2000. Genome Res. 10(10): 1617-1630). Second strand cDNA was primed with the (5'-AGAGAGAGAGCTCGAGCTCTAATAAGGTGACACTATAGAACCA-3') primer. After restriction digestion of the hemimethylated cDNA with BamHI and XhoI, the cDNA was cloned in the lambda FLC-I vector. Subsequently, the library was bulk-excised into pFLC-I plasmid as described (Carninci, P., et al. 2001. Genomics 77(1-2): 79-90). cDNAs were transformed into DH5-alpha TonA strain.

(Stapleton et al., 2002)

Comment

Reported As

Symbol Synonyms

(Stapleton et al., 2002)

RE EST

(Stapleton et al., 2002)

RE_cDNA

Riken embryo library

References (3)

Research paper (2)

Hoskins et al., 2011, Genome Res. 21(2): 182--192

Genome-wide analysis of promoter architecture in Drosophila melanogaster. [FBrf0213090]

Stapleton et al., 2002, Genome Res. 12(8): 1294--1300

The Drosophila Gene Collection: identification of putative full-length cDNAs for 70% of D. melanogaster genes. [FBrf0152058]

Supplementary material (1)

Hoskins et al., 2011, Genome Res. 21(2):

Supplemental Material. [FBrf0213251]

External Crossreferences and Linkouts ( 2 )

Linkouts

DGRC - Stock center for Drosophila cDNAs, vectors, and cell lines

FBcl0211225

Fly-FISH - A database of Drosophila embryo and larvae mRNA localization patterns

RE12101

Synonyms and Secondary IDs (0)

Reported As

Symbol Synonym

Secondary FlyBase IDs

References (0)

Report Sections

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