FB2025_01 , released February 20, 2025
Insertion: Dmel\TI{CRIMIC.TG4.1}SCARCR00797-TG4.1
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General Information
Symbol
Dmel\TI{CRIMIC.TG4.1}SCARCR00797-TG4.1
Species
D. melanogaster
Name
FlyBase ID
FBti0200690
Feature type
insertion_site
Description
Inserted Element
TI{CRIMIC.TG4.1}
LINE ID

CR00797

Affected gene(s)
SCAR
Viability / fertility
Associated allele(s)
SCARCR00797-TG4.1, Scer\GAL4SCAR-CR00797-TG4.1
Stock availability
1 publicly available
Genomic Location
Chromosomal Location
2L ( 32C1 )
Sequence Location
2L:10,978,735..10,978,756 [+]
Target / Docking site
Genomic Maps
Member of Large Scale Dataset(s)
Dataset
CRIMIC-TG4
Description

A set of stocks that each contain a Trojan-GAL4 gene trap sequence in a coding intron, inserted via CRISPR/Cas9-induced homology directed repair. The inserted cassette contains a 'Trojan GAL4' gene trap element composed of a splice acceptor site followed by the T2A peptide, the GAL4 coding sequence and an SV40 polyadenylation signal. When inserted in a coding intron in the correct orientation, the cassette should result in truncation of the trapped gene product and expression of GAL4 under the control of the regulatory sequences of the trapped gene. Each line contains one of three versions of the cassette (TI{CRIMIC.TG4.0}, TI{CRIMIC.TG4.1} or TI{CRIMIC.TG4.2}), depending on the frame required to generate a gene trap. In addition, the presence of inverted attP sites flanking the inserted DNA allows for the entire cassette to be replaced with DNA from a compatible donor plasmid (where the sequence to be inserted is flanked by inverted attB sites) through recombination-mediated cassette exchange (RMCE) driven by the phiC31:int integrase.

(Lee et al., 2018)
Detailed Mapping Data
Chromosome (arm)
Sequence Location
2L:10,978,735..10,978,756 [+]
(Levis, 2018.8.30)
Orientation

+

(Levis, 2018.8.30)
Cytological location (computed by FlyBase)
32C1 (inferred by FlyBase from sequence location)
Cytological location (reported)
32C1_r6 (reported as inferred from sequence location)
(Levis, 2018.8.30)
Insertion into Natural transposon
Comments concerning location

The homology arms of the donor plasmid used in generating the TI{CRIMIC.TG4.1}SCARCR00797-TG4.1 insertion were designed such that there is a small gap between the 3' end of the 5' arm and the 5' end of the 3' arm, thus the insertion is predicted to be accompanied by a deletion of 21bp of genomic sequence flanking the insertion site.

(Levis, 2018.8.30)
Sequence Data
Flanking sequence
Inserted Element
Construct
TI{CRIMIC.TG4.1}
(Lee et al., 2018)
Size (Kb)
Component Allele(s)
Molecular map
Affected Gene(s)
Insertion may affect gene
SCAR
(Gene Disruption Project members, 2018-, Levis, 2018.8.30)
Variant Molecular Consequences
Phenotypic Data
Expression Data
Reporter Expression
Additional Information
Statement
Reference
 
Marker for
Reflects expression of
Reporter construct used in assay
Data on Genetic Line
Line ID

CR00797

(Lee et al., 2018, Levis, 2018.8.30)
Origin as a multiple insertion line
Progenitor(s) within the Genome
Related Aberration or Balancer
Aberration
Balancer
Stocks (1)
External Crossreferences and Linkouts ( 1 )
Linkouts
GDP-CRIMIC
  • CR00797
Synonyms and Secondary IDs (1)
Reported As
Symbol Synonym
TI{CRIMIC.TG4.1}SCARCR00797-TG4.1
(Levis, 2018.8.30)
Name Synonyms
Secondary FlyBase IDs
    References (3)