pReporter_ZF1_ZF2_mNeonGreen
(Plasmid #213836)

• Purpose: Facilitates genomic integration of the reporter for screen 3: ZF-2 followed by ZF-1 upstream of the reporter gene.
• Depositing Lab: James Collins
• Publication: Alcantar et al Molecular Cell, June 2024

Backbone

• Vector backbone: pLEU
• Vector type: Yeast Expression
• Selectable markers: LEU2

Growth in Bacteria

• Bacterial Resistance(s): Spectinomycin, 50 μg/mL
• Growth Temperature: 37°C
• Growth Strain(s): NEB Stable
• Copy number: High Copy

Gene/Insert

• Gene/Insert name: mNeonGreen
• Species: Synthetic

Cloning Information

• Cloning method: Restriction Enzyme
• 5′ cloning site: Unknown (unknown if destroyed)
• 3′ cloning site: Unknown (unknown if destroyed)

Resource Information

• Supplemental Documents:
  • pReporter_ZF1_ZF2_mNeonGreen.gb

Terms and Licenses

• Academic/Nonprofit Terms:
  • UBMTA
  • mNeonGreen Label License
• Industry Terms:
  • Not Available to Industry

Depositor Comments

Contains a minimal CYC1 promoter driving expression of mNeonGreen. Binding sites for ZF-1 (ZF 43-8) and ZF-2 (ZF 42-10) are upstream of the promoter.

Cut with NotI prior to transformation into yeast to facilitate genomic insertion.

**This plasmid is prone to recombination due to ZF binding site repeats.**

How to cite this plasmid

• For your Materials & Methods section:

  pReporter_ZF1_ZF2_mNeonGreen was a gift from James Collins (Addgene plasmid # 213836 ; http://n2t.net/addgene:213836 ; RRID:Addgene_213836)

• For your References section:

  A high-throughput synthetic biology approach for studying combinatorial chromatin-based transcriptional regulation. Alcantar MA, English MA, Valeri JA, Collins JJ. Molecular Cell, June 2024 10.1016/j.molcel.2024.05.025