Tagging and Truncation of TDP1 and PRMT5

Human flag-tagged full-length TDP1 (FLAG-TDP1^WT), His-tagged and green fluorescent protein (GFP)-tagged TDP1 constructs were described previously (10 (link),19 (link)). The FLAG-PRMT5 fusion construct was a kind gift from Dr Shilai Bao (Institute of Genetics and Developmental Biology, CAS, China). The flag-tagged N-terminal (1–293 aa) and C-terminal (294–637 aa) truncated PRMT5 and GFP-tagged N-terminal (1–185 aa) truncated TDP1 constructs were generated by polymerase chain reaction amplification using full-length PRMT5 or full-length TDP1 (FLAG-TDP1^WT) as template and were cloned in the mammalian expression vectors pCMV-Tag2 (Stratagene, La Jolla, CA, USA) or pEGFP-N2 vector (CLONTECH) respectively. The following point mutations: TDP1^R361K, TDP1^R586K, TDP1^{R361K, R586K} in FLAG and GFP tagged TDP1 constructs as well as His-TDP1^R361K,R586K were created using the ‘QuickChange’ protocol (Stratagene, La Jolla, CA, USA). All PCR-generated constructs were confirmed by DNA sequencing.

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Rehman I., Basu S.M., Das S.K., Bhattacharjee S., Ghosh A., Pommier Y, & Das B.B. (2018). PRMT5-mediated arginine methylation of TDP1 for the repair of topoisomerase I covalent complexes. Nucleic Acids Research, 46(11), 5601-5617.

Publication 2018

pEGFP-N2 vector

Green fluorescent protein Human Mammalian Point mutations Protein n Vector

Corresponding Organization : Center for Cancer Research

Other organizations : Indian Association for the Cultivation of Science

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Variable analysis

independent variables

FLAG-TDP1^WT
His-tagged TDP1 constructs
GFP-tagged TDP1 constructs
FLAG-PRMT5 fusion construct
FLAG-tagged N-terminal (1–293 aa) and C-terminal (294–637 aa) truncated PRMT5
GFP-tagged N-terminal (1–185 aa) truncated TDP1
TDP1^R361K
TDP1^R586K
TDP1^R361K,R586K
His-TDP1^R361K,R586K

dependent variables

Not explicitly mentioned

control variables

Not explicitly mentioned

controls

Positive control: None mentioned
Negative control: None mentioned

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