GRNA Production: Difference between revisions

Latest revision as of 12:16, 26 July 2018

(1) Oligo Rehydration

100 μmol [ ] (stock) of oligos

Ex. 100 μmol [ ] —> 27.8 nmol [ ] —> rehydrate oligo bead with 278 μl of H2O

add H2O to hydrate oligos
incubate 5 min at room temp
mix
incubate another 5 min to fully dissolve store at -20°C

(2) Sense / Antisense Oligo Annealation

TRIS Buffer

sufficient to allow oligos to anneal
proper pH (7.5-8)
10 mmol TRIS

2 μl sense oligo, 2 μl antisense oligo, 46 μl TRIS buffer (10 mmol) ————————— 50 μl final vol

incubate samples at high temp to low temp (about -1°C / sec) - must reach 95°C
store at 4°C

(3) Plasmid Digestion

Plasmid DR274 - digest with restriction enzyme BsaI

Always mix then centrifuge reaction components after removing from -20°

Reaction Mix (Add in parenthetical order.)

14.5μl H2O
1μl plasmid DNA (1-2 μg) (1.419 μg/μl —> just use 1 μl)
2μl Buffer IV (10x)
2μl BSA (10x)
10U/μl BsaI (0.5 μl for example)

——————————

20 μl final volume

(4) Gel- Plasmid Digestion

Gel Digestion

1.5% agarose gel
20 μl digestion vol + 3 μl loading dye
run for 40 min @ 130 V
take picture quickly! (avoid excessive UV exposure to nucleic acid)

(5) Gel- DNA Extration/Purification of Plasmid

DNA Extraction Kit (Gel Extraction) weigh eppendorf mct tube — slice out band from gel

place in tube
weigh again
add volume of Buffer 1 equivalent to weight difference (gel slice weight) — incubate at 60°C for 5-10 min to let gel dissolve in extraction buffer

(should look yellow. pink/red means too basic)

apply solution to column
incubate for 1 min
centrifuge @ 13,000 rpm, 1 min
put column back to the original tube
add 500 μl wash B (salt + EtOH)
centrifuge 13,000 rpm 1-1.5 min
put column back in column tube
centrifuge @ 13,000 rpm, 2 min
put column into new 1.5 mL Eppendorf microcentrifuge tube — add 20ul H2O to column
incubate 1 min
centrifuge @ 13,000 rpm, 1 min
add 20ul H2O to column
incubate 1 min
centrifuge @ 13,000 rpm, 1min

(6) gRNA oligo ligation into plasmid

Reaction Mix

3μl sense/antisense annealed oligos
1μl purified vector (Kan. resistant)
1μl 10x Buffer (salts, ATP, DTT, etc.)
0.5μl ligase
4.5μl H2O

——————————

10μl final vol

Master Mixes (when doing many ligations simultaneously)

(1) Master Mix #1 (mix then pipette into PCR tubes)

1 μl Vextor x (n+1)
0.8 μl 10x BF x (n+1)
3.2 μl H2O (n+1)

————————

5 μl / PCR tube final vol

3 μl of oligo (pipette directly into PCR tubes with MM#1)

Master Mix #2 (mix then pipette into PCR tubes)

0.5μl enzyme x (n+1)
0.2μl 10x BF x (n+1)
1.3μl H2O x (n+1)

————————————

2 μl / PCR tube

4° C ON

(7) Transformation

Use recombinant bacterial cells, strain DH5α (e. coli substrain) (in PCR tubes in -80°) - must ALWAYS keep on ice!!
4μl aliquot (ligation product) into common mix (-80C°) (~20-30 μl in common mix)
incubate on ice for 25 min
heat change —> 42°C in 1.5 min
incubate on ice for 3.5 min
put into Eppendorf w/ LB (no antibiotics - give cells a chance to express the plasmid gene against antibiotics)
culture at 37°C for 1 hr
centrifuge: 6,000 rpm / 1min
trash most supernatant
resuspend e. coli culture (w/ leftover LB) plate - LB + Kan antibiotics
incubate 37° overnight

Note:

Kan 50 mg/L - high copy

Kan 15 mg/L - low copy

Notes:

If very efficient ligation / transformation with plasmid, then there will be an increased # of colonies that can survive. Therefore you should do a 2x plating (2x plates per transformation) so you can pick single colonies w/o contamination
∴ 2x plates per PCR tube of transformed DH5α — 25 μl / plate —gradient plating
Akira prepares common stock of DH5α for the lab.
Use 4μl ligation product for newly ligated plasmids. If proven highly efficient, use 1μl of product.
42°C incubation - use Jifeng’s ’42 Keep’ thermal cycler program
For Amp. resistance, LB culture is not necessary
For Amp res. plasmids, add 50-100μl of LB directly to PCR tube, then plate
After plating, allow to dry until no excess liquid
Culture in 37° incubator ON (16 hours max!!!) in semi open plastic bag to avoid excessive moisture loss

(8) Miniculture n (number of colonies you want to culture) —> n separate vials / per plate

Culture Solution Kan = 50 mg/mL (stock concentration)

—> 50 mg/L final dilution / concentration

ex. 100 mL PBS + 100 μl Kan

use pipette tip to transfer colony gently to tube (can drop expel pipette tip directly into tube to be removed after centrifugation)
8 hours ON at 37°C

(9) Miniprep Protocol

ON culture
centrifuge 5000 rpm / 10 min discard supernatant
add 250μl P1
resuspend pellet in P1

transfer to 2mL Eppendorf tubes
add 250 μl P2
mix by inverting until solution becomes blue

add 350 μl N3 (guanidine hydrochloride acetyl acid)
mix immediately by inverting tubes until solution (blue) turns colorless
centrifuge 13,000 rpm / 10 min

label QIAprep spin columns
transfer supernatant to QIAprep spin columns
incubate / let stand for 1 min
centrifuge @ 13,000 rpm / 2 min
discard spin-through
+ 750 μl PE to column
centrifuge @ 13,000 rpm / 2 min
+ 750 μl PE to column
centrifuge @ 13,000 rpm / 2 min
vacuum columns’ inner rim/ridge (do NOT vacuum membrane) remove columns
label 1.5mL Eppendorf tubes
places columns into 1.5mL Eppendorf tubes
add 50 μl dH2O
let stand 1 min
centrifuge 1 min
store samples at -20°C

(10) Miniprep Sample Sequencing

Sequencing reaction

2 Kb plasmid

requires ~100 ng [ ] per tube

_____ ng/μl [ ]

ex. 170 ng/μl [ ]

0.7μl sample

4.3μl H2O

for multiple samples around 170ng/μl [ ], use 4.3μl H2O and then add appropriate concentration of sample to sequencing PCR tube
M13_F primer
max read length
check sequences for gRNA inserts

(11) Plasmid gRNA PCR Amplification

Mix 0.2μl sample

0.3μl For

0.3μl Rev

25μl Phusion MasterMix (with NTs and Taq) *** 24.2μl ddH2O

—————————

50 μl total vol

- - 2x Phusion 9c ‘MasterMix’ (Thermo) #F-532

Master Mix

(n + 0.5) x each component
use pipette tips with filters
For + Rev + Phusion MM + ddH2O
label sides + top of tubes (#1 - #n)
briefly centrifuge samples + primers + Phusion (once dissolved)
add For + Rev + Phusion MM + ddH2O into ‘MM’ tube
pipette up and down to mix (~5x times)
aliquot 49.8 μl of MM into each PCR tube
add 0.2 μl sample to each tube
put in / start thermalcycler

(12) QIAquick PCR Purification Kit

5 volumes Buffer PB to 1 vol PCR rxn (add directly to PCR tube)
mix

(if orange or violet, add 10μl 3M sodium acetate and mix)

(mix should turn yellow)

place QIAquick columns in 2mL collection tubes

bindDNA - add sample to column
incubate for 1 min
centrifuge for 30-60 sec
discard flow through + put column back in 2mL tube

wash - add 0.75mL PE to column
centrifuge for 30-60 sec
discard flow-through + put column back in 2 mL tube
centrifuge QIAquick column for 1 min in 2 mL collection tube
vacuum rim of column (10μl tip + 1mL tip + vac system)
centrifuge QIAquick column for 1 min in 2 mL collection tube

place columns in RNase free 1.5mL microcentrifuge tubes (put lids on column tubes and cut the column tubes’ lids off)
eluteDNA - add 20μl RNase free H2O to centre of column centrifuge column for 1 min
measure concentration (nanodrop)

(13) Purified PCR product gel 1μl purified product

1μl dye

5/6 μl TBE (1x)

————————————

8/9 μl total vol

(2μl Red / 50 mL of gel solution)

(14) MEGAscript Kit (amnion / life technologies)

Prep

prepare 70% EtOH - minimum 3mL / sample (for day 2)
keep RNAPol on ice at all times
thaw frozen reagents
vortex 10x RBuffer and NTPs
briefly centrifuge
(NTPs should be kept on ice. 10x RB must be kept at room temp.)

Assemble Txn Rxn

Sample

Use ~500ngof Miniprep sample —> use Nanodrop concentration to calculate volume

MasterMix

Add MM components in the following order: H2O, NTPs, 10x BF, enzyme mix, MPI T7

(n = number of samples + 0.5)

n x 2μl ATP

n x 2μl CTP

n x 2μl GTP

n x 2μl UTP

n x 2μl 10x Buffer

n x ___μl H2O

n x 0.5μl MPIT7 (separate - Max Planck purified T7 enzyme)

n x 2μl Enzyme Mix

___μl MasterMix + ___μl sample = 20μl

add sample volume directly to PCR tubes
add MasterMix to samples
mix thoroughly
incubate in thermalcycler, 37°C, overnight (max 16 hrs.)

Day 2

TURBO DNase

add 1μl TURBO DNase
mix well
incubate further 15 min at 37°C
label RNase free 1.5mL microcentrifuge (μc)tubes

RNA Recovery - LiCl Precipitation

precipitate RNA

add 30μl RNase free H2O
add 30μl LiCl precipitation solution

(preferred method: add LiCl to newly labeled 1.5mL μc tubes, add 30μl H2O to samples, transfer H2O + samples (50μl) to the μC tubes with LiCl) *mix thoroughly

chill >30 min at -20°C
centrifuge: 4°C, max speed, 15 min
CAREFULLY remove supernatant
wash pellet with 1mL 70% EtOH
centrifuge: 4°C, max speed, 15 min
wash pellet with 1mL 70% EtOH
centrifuge: 4°C, max speed, 15 min
wash pellet with 750μl 70% EtOH (lower vol. allows for easier removal of final wash) (3x total washes - centrifuge between each wash)
centrifuge: 4°C, max speed, 15 min
carefully remove EtOH
air dry 5-10 min
resuspend RNA in~50μl RNase free H2O (Variable volume. If some pellets are smaller, use less H2O.) (make very sure pellet is fully resuspended - tricky because appears clear)
determine concentration using Nanodrop (remember to use RNA detection)
store at -80°C

(15) gRNA - Cas9 complex formation

Injection / electroporation complex

10-20μg protein (from prep 5 μg/μl)

5μg each gRNA (concentration dependent)

0.9 μg 10x Cas9 Buffer

__ μl H2O

———————————

10 μl final volume

Microinjection (single cell stage complex)

5μg protein (around 1 μl - from prep 5μg/μl)

4 μg gRNA ([] dependent)

0.9μl 10x Cas9 Buffer

__μl Hzo

1 μl Fastgreen

———————————

10μl final volume

Add in seq.

H2O
Buffer
gRNA
Protein

aliquot 5 ———————————l into 2x 1.5 mL PCR tubes (hyper sterile)
incubate at room temp for 5 min.
store at -80°C

GRNA Production: Difference between revisions

Latest revision as of 12:16, 26 July 2018

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