Standard

Protein trap : a new Swiss army knife for geneticists? / Fedorova, Svetlana A.; Dorogova, Natalya V.

в: Molecular Biology Reports, Том 47, № 2, 02.2020, стр. 1445-1458.

Результаты исследований: Научные публикации в периодических изданияхобзорная статьяРецензирование

Harvard

Fedorova, SA & Dorogova, NV 2020, 'Protein trap: a new Swiss army knife for geneticists?', Molecular Biology Reports, Том. 47, № 2, стр. 1445-1458. https://doi.org/10.1007/s11033-019-05181-z

APA

Fedorova, S. A., & Dorogova, N. V. (2020). Protein trap: a new Swiss army knife for geneticists? Molecular Biology Reports, 47(2), 1445-1458. https://doi.org/10.1007/s11033-019-05181-z

Vancouver

Fedorova SA, Dorogova NV. Protein trap: a new Swiss army knife for geneticists? Molecular Biology Reports. 2020 февр.;47(2):1445-1458. Epub 2019 нояб. 14. doi: 10.1007/s11033-019-05181-z

Author

Fedorova, Svetlana A. ; Dorogova, Natalya V. / Protein trap : a new Swiss army knife for geneticists?. в: Molecular Biology Reports. 2020 ; Том 47, № 2. стр. 1445-1458.

BibTeX

@article{d26372db22bf4e86a5015a329fd43254,
title = "Protein trap: a new Swiss army knife for geneticists?",
abstract = "The protein trap is a powerful tool for genetic and biochemical studies of gene function in the animal kingdom. Although the original protein trap was developed for flies, it can be easily adapted to other multicellular organisms, both known models and ones with an unsequenced genome. The protein trap has been successfully applied to the fruit fly, crustaceans Parhyale hawaiensis, zebrafish, and insect and animal cell cultures. This approach is based on the integration into genes of an artificial exon that carries DNA encoding a fluorescent marker, standardized immunoepitopes, an integrase docking site, and splice acceptor and donor sites. The protein trap for cell cultures additionally contains an antibiotic resistance gene, which facilitates the selection of trapped clones. Resulting chimeric tagged mRNAs can be interfered by dsRNA against GFP (iGFPi—in vivo GFP interference), or the chimeric proteins can be efficiently knocked down by deGradFP technology. Both RNA and protein knockdowns produce a strong loss of function phenotype in tagged cells. The fluorescent and protein affinity tags can be used for tagged protein localisation within the cell and for identifying their binding partners in their native complexes. Insertion into protein trap integrase docking sites allows the replacement of trap contents by any new constructs, including other markers, cell toxins, stop-codons, and binary expression systems such as GAL4/UAS, LexA/LexAop and QF/QUAS, that reliably reflect endogenous gene expression. A distinctive feature of the protein trap approach is that all manipulations with a gene or its product occur only in the endogenous locus, which cannot be achieved by any other method.",
keywords = "Chimeric protein, Gene expression, Intracellular markers, Protein trap, Recombinant proteins, RMCE, RNAi, Trap conversion",
author = "Fedorova, {Svetlana A.} and Dorogova, {Natalya V.}",
year = "2020",
month = feb,
doi = "10.1007/s11033-019-05181-z",
language = "English",
volume = "47",
pages = "1445--1458",
journal = "Molecular Biology Reports",
issn = "0301-4851",
publisher = "Springer Netherlands",
number = "2",

}

RIS

TY - JOUR

T1 - Protein trap

T2 - a new Swiss army knife for geneticists?

AU - Fedorova, Svetlana A.

AU - Dorogova, Natalya V.

PY - 2020/2

Y1 - 2020/2

N2 - The protein trap is a powerful tool for genetic and biochemical studies of gene function in the animal kingdom. Although the original protein trap was developed for flies, it can be easily adapted to other multicellular organisms, both known models and ones with an unsequenced genome. The protein trap has been successfully applied to the fruit fly, crustaceans Parhyale hawaiensis, zebrafish, and insect and animal cell cultures. This approach is based on the integration into genes of an artificial exon that carries DNA encoding a fluorescent marker, standardized immunoepitopes, an integrase docking site, and splice acceptor and donor sites. The protein trap for cell cultures additionally contains an antibiotic resistance gene, which facilitates the selection of trapped clones. Resulting chimeric tagged mRNAs can be interfered by dsRNA against GFP (iGFPi—in vivo GFP interference), or the chimeric proteins can be efficiently knocked down by deGradFP technology. Both RNA and protein knockdowns produce a strong loss of function phenotype in tagged cells. The fluorescent and protein affinity tags can be used for tagged protein localisation within the cell and for identifying their binding partners in their native complexes. Insertion into protein trap integrase docking sites allows the replacement of trap contents by any new constructs, including other markers, cell toxins, stop-codons, and binary expression systems such as GAL4/UAS, LexA/LexAop and QF/QUAS, that reliably reflect endogenous gene expression. A distinctive feature of the protein trap approach is that all manipulations with a gene or its product occur only in the endogenous locus, which cannot be achieved by any other method.

AB - The protein trap is a powerful tool for genetic and biochemical studies of gene function in the animal kingdom. Although the original protein trap was developed for flies, it can be easily adapted to other multicellular organisms, both known models and ones with an unsequenced genome. The protein trap has been successfully applied to the fruit fly, crustaceans Parhyale hawaiensis, zebrafish, and insect and animal cell cultures. This approach is based on the integration into genes of an artificial exon that carries DNA encoding a fluorescent marker, standardized immunoepitopes, an integrase docking site, and splice acceptor and donor sites. The protein trap for cell cultures additionally contains an antibiotic resistance gene, which facilitates the selection of trapped clones. Resulting chimeric tagged mRNAs can be interfered by dsRNA against GFP (iGFPi—in vivo GFP interference), or the chimeric proteins can be efficiently knocked down by deGradFP technology. Both RNA and protein knockdowns produce a strong loss of function phenotype in tagged cells. The fluorescent and protein affinity tags can be used for tagged protein localisation within the cell and for identifying their binding partners in their native complexes. Insertion into protein trap integrase docking sites allows the replacement of trap contents by any new constructs, including other markers, cell toxins, stop-codons, and binary expression systems such as GAL4/UAS, LexA/LexAop and QF/QUAS, that reliably reflect endogenous gene expression. A distinctive feature of the protein trap approach is that all manipulations with a gene or its product occur only in the endogenous locus, which cannot be achieved by any other method.

KW - Chimeric protein

KW - Gene expression

KW - Intracellular markers

KW - Protein trap

KW - Recombinant proteins

KW - RMCE

KW - RNAi

KW - Trap conversion

UR - http://www.scopus.com/inward/record.url?scp=85075069830&partnerID=8YFLogxK

U2 - 10.1007/s11033-019-05181-z

DO - 10.1007/s11033-019-05181-z

M3 - Review article

C2 - 31728729

AN - SCOPUS:85075069830

VL - 47

SP - 1445

EP - 1458

JO - Molecular Biology Reports

JF - Molecular Biology Reports

SN - 0301-4851

IS - 2

ER -

ID: 22344531