Team:MIT/miRNA Group Notebook protocols old data

LR Reaction (4/1/2016, Liz, Wangui, Maya) · Benchling

LR Reaction (4/1/2016, Liz, Wangui, Maya)

Introduction

An LR reaction insertd one or more parts in pENTR vectors into pDEST vector. Used to assemble transcriptional units from promoters and genes.

Materials

  • Promoter pENTER plasmif: L4-Promoter-R1
    • Working concentration: 5 fmol/ul
  • Gene pENTR plasmid: L1-Gene-L2
    • Working concentration: 5 fmol/ul
  • Destination plasmid: pDEST
    • Working concentration: 5 fmol/ul
  • 200 ul PCR strip tubes, 1 tube per rxn ( 3 tubes)
    • 5x LR Clonase II
      • Stored in ~5 ul liquots in the -80 in room 235. Don't remove an aliquot until you're ready to use it.
    • Proteinase K
      • Stored in ~5 ul liquots in the -80 in room 235. Don't remove an aliquot until you're ready to use it.

    Procedure

    • LR Reaction Setup
    1. For each LR you are doing, fill out a column in the following tabe:
    A
    B
    C
    D
    1
    		Tube LabelTETTHR
    2
    		Promoter pENTRpTal14pTREhef1a
    3
    		Gene pENTRmEYFPTal14rtTA
    4
    		pDEST
    5
    		LizWanguiMaya
    Table1
    1. For each LR, label a 200 ul strip tube with your initials and tube number.
    1. Into each tube, pipette:
    • -- 1 ul of promoter pENTR
    • -- 1 ul of the gene pENTR
    • -- 2 ul of the pDEST
    1. Retrieve an aliquot of LR Clonase from the -80
    • Bring an razor blade with you, you'll need to cut s tube from the strip tubes
    1. Pulse the LR clonase tube in the microfuge to collect the clonase at the bottom
    1. Add 1 ul of the LR clonase to each LR reaction.
    1. Cap the tubes.
    1. Flick them several times to mix.
    1. Pulse-spin the tubes in the microfuge to collet the liquid at the bottom.
    1. Incubate at room temperature for at least 12 hours and not more than 24 hours. (Started incubation at 4:30pm)
    • A popular strategy is to tape the tubes to the shelves over the bench, with your initials and date
    • 16-24 Hours later: Proteinase K kill (Saturday 10am)
    1. Retrieve a 5 aliquot of peoteinase K from the -80 freezer
    1. That in your fingers, then pulse in the microfuge to collect at the bottom of the tube
    1. Pipette 1 ul into each of the LR reations
    1. Flick serveral times to mix
    1. Pulse-spin the tubes in the microcentrifuge
    1. Incubate at 37 degrees Celsius for 15 minutes, or room-temperature for an hour:
    • PAUSE POINT: You can store the reactions in the -20 indefinitely until the transformation
    00:10:00
    1. Proceed to transformation. Transform 2 ul. (Sunday 3pm)
    Lipofectamine 2000 Optimization for DNA · Benchling

    Lipofectamine 2000 Optimization for DNA

    Made with Benchling
    Project: miRNA and Repressors subgroup
    Authors: Wangui Mbuguiro
    Dates: 2016-08-04 to 2016-08-12
    Thursday, 8/4
    Done in tHESC --> Scroll down to 2.0, Julia
    Transfection marker: hef1a:mKate (109 ng/ul)
    Reagent: Lipofectamine 2000
    Independent Variable: Amount of Lipofectamine 2000 (1.0uL, 1.5 uL, 2.0 uL, 2.5 uL)
    Dependent Variable: Amount of fluorescene
    Control: Amount of DNA (500ng per well), 24 Well plate
    Well 1: 1.0 uL lipofectamine
    Well 2: 1.5 uL
    Well 3: 2.0 uL
    Well 4: 2.5 uL
    Well 5: 1.0 uL lipofectamine '
    Well 6: 1.5 uL '
    Well 7: 2.0 uL'
    Well 8: 2,5 uL'
    Well 9: untransfected
    Dilute lipofectamine 2000 reagent in opti-mem until total volume 50uL
    Dilute DNA in opti-mem until total volume 50 uL
    Wait 5 mins.
    Combine 25uL of DNA and lipofectamine dilutions into one tube and incubate for 20 minutes.
    Add the 50uL of DNA+Lipofectamine complex to seeded wells.
    Setup:
    Eppendorf tubes
    Lipofectamine tubes:
    2 uL Lipofectamine, 48 uL opti-mem
    3 uL Lipofectamine, 47 uL opti-mem
    4 uL Lipofectamine, 46 uL opti-mem
    5 uL Lipofectamine, 45 uL opti-mem
    DNA (hef1a:mKate) tubes:
    10 uL hef1a:mKate, 40 uL opti-mem X 4
    Checked 3 hours later: No fluorescence
    Cyto Flo Results: Minial to no transfection
    Friday, 8/12
    Lipofectamine 2000 DNA Transfection Optimzation 2.0
    Transfection marker: hef1a:mKate (109 ng/ul)
    Reagent: Lipofectamine 2000
    DNA: ANY (except hef1a:mKate). Could dilute to 100 ng/ul for ease
    Independent Variable: Amount of Lipofectamine 2000 (3.0uL, 4 uL, 5 uL, 6 uL)
    Dependent Variable: Amount of fluorescene
    Well 1: 3.0 uL lipofectamine
    Well 2: 4.0 uL
    Well 3: 5.0 uL
    Well 4: 6.0 uL
    Well 5: untransfected
    Dilute lipofectamine 2000 reagent in opti-mem until total volume 50uL
    Dilute DNA in opti-mem until total volume 50 uL
    Wait 5 mins.
    Combine 25uL of DNA and lipofectamine dilutions into one tube and incubate for 20 minutes.
    Add the 50uL of DNA+Lipofectamine complex to seeded wells.
    Setup:
    Eppendorf tubes
    Lipofectamine tubes:
    6 uL Lipofectamine, 44 uL opti-mem
    8 uL Lipofectamine, 42 uL opti-mem
    10 uL Lipofectamine, 40 uL opti-mem
    12 uL Lipofectamine, 38 uL opti-mem
    DNA (hef1a:mKate) tubes:
    10 uL hef1a:mKate, 40 uL opti-mem X 4
    Making SOC · Benchling

    Making SOC

    Introduction

    SOC = SOB ("Super Optimal Broth") + Glucose (@40% w/v) Brian advised having SOB0 autoclaved first, and then adding glucose to SOB using a vacuum + filter with proper aseptic technique. If you end up making SOC, please write up detailed procedures, so other people can too :)

    Materials

    • SOB
      • In coldroom or on bench
    • 40% Glucose
      • Above bench or ask Brian

    Procedure

    • Dilute 40% glucose to 2% using SOB (1:20)
    1. Use a sterile bottle (same kind that 40% glucose in)
    1. This can be done at the bench
    Midiprep · Benchling

    Midiprep

    Introduction

    Purifying large amount of DNA to tranfect mammalian cells

    Materials

    • Qiagen MidiPrep

    Procedure