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GrainGenes Sequence Report: BF257986

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Sequence
BF257986
External Databases
Data at GenBank
Data at EMBL
Data at DDBJ
NCBI UniGene
Hv.22943
DB Remark
Locus Source: Hordeum vulgare subsp. vulgare
UniGene title 'CDNA clone: FLbaf118j14, mRNA sequence'
Keyword
EST
Species
Hordeum vulgare subsp. vulgare
Cultivar
Morex
Clone Library
Hordeum vulgare seedling root EST library HVcDNA0007 (Etiolated and unstressed)
Tissue
Seedling root
Data Source
genbankRelease 135, Apr 15 2003
genbankUpdated Nov 2006
Title
HVSMEf0014G19f Hordeum vulgare seedling root EST library HVcDNA0007 (Etiolated and unstressed) Hordeum vulgare subsp. vulgare cDNA clone HVSMEf0014G19f, mRNA sequence.
Strain
lab_host TJC121
vulgare
Clone
HVSMEf0014G19f
Probe
[Bcl2ct2cn6]
{SpCl-25}
BF257986
Remark
DB_xref: taxon:112509
Feature: source: mol_type = 'mRNA';
Locus Comment: On Nov 16, 2000 this sequence version replaced gi:11187099.; Contact: Wing RA; Clemson University Genomics Institute; Clemson University; 100 Jordan Hall, Clemson, SC 29634, USA; Tel: 864 656 7288; Fax: 864 656 4293; Email: rwing@clemson.edu; Total hq bases = 209; Seq primer: AATTAACCCTCACTAAAGGG; High quality sequence start: 2; High quality sequence stop: 387.
Note: Vector: lambdaZAP; Site_1: EcoR1; Site_2: Xho1; Seeds were surface sterilized then germinated under axenic conditions in the dark at room temperature on filter paper with water, nystatin and cefotaxime in covered crystallization dishes. Five-day old seedling roots were then harvested, total RNA was prepared, poly(A) RNA was purified, one primary unamplified cDNA library was made, and 1 million pfu were in vivo excised to give pBluescript SK(-) cDNA phagemids. These steps were performed in the TJ Close laboratory at the University of California, Riverside (Choi, Close, Fenton). Phagemids were plated and picked at the Clemson University Genomics Institute (CUGI) (Begum, Palmer, Frisch, Atkins and Wing). Plasmid DNA preparations, DNA sequencing and sequence analysis were performed at CUGI (Wing, Yu, Frisch, Henry, Simmons, Oates , Rambo, Main). The sequence has been trimmed to remove vector sequence and contains a minimum of 100 bases of phred value 20 or above. For more details on library preparation and sequence analysis see http:
Note: Vector: lambdaZAP; Site_1: EcoR1; Site_2: Xho1; Seeds were surface sterilized then germinated under axenic conditions in the dark at room temperature on filter paper with water, nystatin and cefotaxime in covered crystallization dishes. Five-day old seedling roots were then harvested, total RNA was prepared, poly(A) RNA was purified, one primary unamplified cDNA library was made, and 1 million pfu were in vivo excised to give pBluescript SK(-) cDNA phagemids. These steps were performed in the TJ Close laboratory at the University of California, Riverside (Choi, Close, Fenton). Phagemids were plated and picked at the Clemson University Genomics Institute (CUGI) (Begum, Palmer, Frisch, Atkins and Wing). Plasmid DNA preparations, DNA sequencing and sequence analysis were performed at CUGI (Wing, Yu, Frisch, Henry, Simmons, Oates, Rambo, Main). The sequence has been trimmed to remove vector sequence and contains a minimum of 100 bases of phred value 20 or above. For more details on library preparation and sequence analysis see http:
DNA
cgcatcgccaccttccttcctccctccctccctccctccctcgccatctc
cgacccgggttgcggccaatggcggaccagctcaccgacgaccagatcgc
cgagttcaaggaggctttcagcctcttcgacaaggatggggacggttgca
ttacgaccaaggagctgggaactgtcatgcgttccctggggcagaatccc
actgaggcagagctgcaagacatgatcaatgaagtggatgccgacggcaa
tggaacaattgatttccccgaattcctcaaccttatggcccgcaagatga
aggacactgattctgaggaagagctcaaggaggcattccgtgtgttcgac
aaggatcaaaatggttttatctctgctgctgaactgcgccatggtctgac
ccaccttggggagaagttgactgatgaggacggtgaccaatatgatccgc
gagggctgagttgatggcgacgggcagatcaactatgacgaaatttggta
aagtcatgaaggcccaacgaagtggcattaccatctgaagggaagccctc
ggtgttaaaaccaacaaatgaaccc

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