Tetracycline-Inducible Plasmid Construction

A tetracycline inducible promoter was designed with a CMV minimal promoter, a human ubiquitin promoter and a reverse transactivator sequence (ThermoFisher Scientific). The sequence was flanked with AscI and NotI restriction sites and was cloned into the plasmid PCI ASCI, which is our previously described PCI plasmid^{15 (link)} with an AscI cut site upstream of the CMV promoter. The new construct is designated PCI ASCI TET. MR1GFP was ligated into this construct using EcoRI and KpnI to create TET-MR1GFP. Confirmatory sequencing was performed. Restriction enzymes and ligation kit were obtained from New England Biolabs. PCR and gel purification kits were obtained from Qiagen. Transfection of TET-MR1GFP was done using an Amaxa Nucleofector, Kit T solution (Lonza). Each transfection reaction was done with 1e6 cells and 6 µg of TET-MR1GFP plasmid.

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Karamooz E., Harriff M.J., Narayanan G.A., Worley A, & Lewinsohn D.M. (2019). MR1 recycling and blockade of endosomal trafficking reveal distinguishable antigen presentation pathways between Mycobacterium tuberculosis infection and exogenously delivered antigens. Scientific Reports, 9, 4797.

Publication 2019

Restriction enzymes ligation kit PCR and gel purification kits

Cells Ecori Human ubiquitin Ligation Plasmid Restriction enzymes Tetracycline Transactivator Transfection

Corresponding Organization : VA Portland Health Care System

Other organizations : Oregon Health & Science University

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Variable analysis

independent variables

Tetracycline inducible promoter design
Cloning of the promoter construct into the PCI ASCI plasmid
Ligation of MR1GFP into the TET-MR1GFP construct

dependent variables

Expression of MR1GFP

control variables

AscI and NotI restriction sites used for cloning
EcoRI and KpnI used for ligation of MR1GFP
Restriction enzymes and ligation kit from New England Biolabs
PCR and gel purification kits from Qiagen
Transfection using Amaxa Nucleofector, Kit T solution (Lonza)
Transfection with 1e6 cells and 6 µg of TET-MR1GFP plasmid

controls

Positive control: Not explicitly mentioned
Negative control: Not explicitly mentioned

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