Latest revision as of 03:55, 22 October 2019

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PROTOCOLS

PROTOCALS

I.Endogenous transcription factor(TF) selection （Bioinformatics）

screen for highly expressed genes in tumor groups in all invasive breast cancer from GEPIA database. Then, 245 genes is selected initially.
86 normal breast transcriptome samples and 303 tumor transcriptome samples were downloaded from TCGA (The Cancer Genome Atlas) database. The differentially expressed genes were screened by EdgeR algorithm. And all genes were selected in the GEPIA results set (245).
Using the GEPIA database to test the most specific differential gene in invasive breast cancer, and finding out that 11 overlaps with the previously selected 245 in PART 2.
Set priority order for transcription factor identification. Finally, 9 transcription factors were identified

II.mRNA qPCR

1.Reverse Transcription for mRNA

Step One 12μl	Water	10μl
	RNA	1mg
	Random Primer	1μl
	Operate the PCR instrument at 65℃ for 5min and put on ice immediately after taking it out
Step Two 8μl	5X Reaction Buffer	4μl
	Rib RNase Inhibitor	1μl
	10Mμ dNTP mix	2μl
	Reversed Aid RT	1μl
Total:20μl

Then operate the PCR instrument：25℃ 5min→42℃ 60min→70℃ 5min→4℃ ∞

2.qPCR of cDNA obtained from miRNA RT reaction

SYBR	5μl
F Primer	0.2μl
R Primer	0.2μl
ddH₂O	2.6μl
cDNA	2μl
Total	10μl
Then put them for qPCR machine
95℃ for 10min
95℃ for 15s	40 cycles
60℃ for 60s	40 cycles
4℃ reserved

III.miRNA series methods

1.RT Reaction for microRNA

1.1 Preparing for RT Reaction Mix

In a 1.5ml microcentrifuge tube , prepare RT Reaction Mix according to the following table:

Component	Volume (1 reaction)	Volume (10 reactions)
100mM dNTPs (with dTTP)	0.15μl	1.65μl
MultiScribe^TM Rerverse Transcriptase , 50U/μl	1.00μl	11.00μl
10X Reverse Transcription Buffer	1.50μl	16.50μl
RNase Inhibitor , 20U/μl	1.50μl	16.50μl
Nuclease-free Water	4.16μl	45.76μl
Total RT Reaction Mix volume	7.00μl	77.00μl

Place the RT Reaction Mix on ice, then immediately proceed as followed procedures

Primer(RT) design：stem loop method

1.2 Performing reverse transcription

Combine 3μl of 5X RT Primer and 5 μl of double-stranded template in a reaction tube.
Mix thoroughly, then centrifuge briefly to collect the contents at the bottom of the tube.
Incubate at 85℃ for 5min
Incubate at 60℃ for 5min, then place on ice
Add 7μl of RT Reaction Mix to each reaction tube. (details from “Preparing for RT Reaction Mix” showed above)
Centrifuge briefly to collect the contents at the bottom of the tubes

Place on ice and proceed immediately to “Performing reverse transcription” below.

1.3 Performing reverse transcription

Place the reaction tubes into a thermal cycler, then incubate using standard cycling, a reaction volume of 15.0μl, and the following settings.

Step	Temperature	Time
Reverse transcription	16℃	30min
Reverse transcription	42℃	30min
Stop reaction	85℃	5min
Hold	4℃	Hold

The RT reaction products are stored at -25℃

2.qPCR of cDNA obtained from microRNA reverse transcription

SYBR	5μl
F Primer	0.2μl
R Primer	0.2μl
ddH₂O	2.6μl
cDNA	2μl
Total	10μl
Then put them for qPCR machine
95℃ for 10min
95℃ for 15s	40 cycles
60℃ for 60s	40 cycles
4℃ reserved

IV.Sponge

1.PCR for Sponge

Reagent	Volume(μl)
5X Buffer	10
DMSO	4
dNTP	4
Forward Primer	2
Reverse Primer	2
Targeted DNA fragment	1
phusion	1
ddH₂O	26
In Total	50

Then put the reaction system to the PCR machine

Cycle	Temperature	Time
	94℃	5min
10 cycles Add 0.5℃ after per cycle	94℃	30s
	55℃	30s
	72℃	30s
25 cycles	94℃	30s
	60℃	30s
	72℃	30s
	72℃	7min
	4℃	reserved

V.miRNA-BS

1.PCR for Binding site（BS）

	94℃	5min
10 cycles Add 0.5℃ after per cycle	94℃	30s
	55℃	30s
	72℃	30s
25 cycles	94℃	30s
	60℃	30s
	72℃	30s
	72℃	7min
	4℃	reserved

2.Digestion of Binding site（BS）

BS-1	20μl
BS-2	20μl
Bbs1	2μl
10XBuffer	5μl
ddH₂O	6μl
Total	50μl

Examples:

BS-1: miR141-BS

BS-2: miR148-b-BS

VI.Double digestion to construct plasmid

1.Digestion

	DNA	Vector
In Total	10	15
Kpn1	1	1
Xho1	1	1
10XBuffer	2	2
ddH₂O	6	11

2.Connection

Fragment	3μl
Vector	10μl
10XBuffer	2μl
T₄ DNA Ligase	3μl
ddH₂O	2μl
Total	20μl

VII.Golden Gate methods

1.Goldengate splicing

Example that synthase Module2: making s(ESR1)p and Sponge connected

Vector	2μl
Sponge	1μl
s(ESR1)p	1μl
10XT₄ Ligase Buffer	2μl
10XBuffer	2μl
Esp3L	1μl
ddH₂O	11μl
Total	20μl

2.PCR amplification

Step 1(X10)
37℃	5min
16℃	10min
Step 2
37℃	15min
50℃	5min
80℃	5min
Step 3
16℃	reserved

Then the 10mM ligation was chemically transformed, screened and cloned by blue and white method, and the positive clones were made into colony PCR and sent for sequencing

VIII.Luciferase assay

1.Measurement of Luciferase

discard the medium with Luciferase plasmid 48h after transfection and wash it with PBS
add 1XL_ys Buffer 50 mu/hole (diluted from 5XL_ys Buffer)
freeze at -80℃ for 30 minutes
take out, natural melting on ice, centrifuge set 4℃ ready
take out the precooled ep tube and scrape the cells with tip head to transfer the cells into the ep tube
13,000g centrifuge for 10min, set aside

Detection: take a new ep tube, add 20 microns luciferase detection reagent (stored at -80℃), add 10 microns to each tube to get the supernatant, mix evenly, and test under the enzyme label meter.

2.Measurement of LacZ

discard the medium with Luciferase plasmid 48h after transfection and wash it with PBS
add 1XL_ys Buffer 50 mu/hole (diluted from 5XL_ys Buffer)
freeze at -80℃ for 30 minutes
take out, natural melting on ice, centrifuge set 4℃ ready
take out the precooled ep tube and scrape the cells with tip head to transfer the cells into the ep tube
13,000g centrifuge for 10min, set aside

Detection:

a. Take 96-well plates and add 100 micron LacZ Buffer into each hole

b. The supernatant obtained by adding 10 microns per hole

c. The temperature of 37 ℃) for 30 min

d. When the sample turned yellow, 50 micron l 1 micron NaCO*10HO was added to terminate the reaction232

e. LacZ was detected with microplate reader, wavelength =405nm

IX.Cell Biological protocols

1.Cell planking

the medium
wash it with PBS (1~2ml)
trypsin (1ml) can be digested in the 40s to 1990s, during which time it can be placed in the incubator
add 5ml medium to terminate digestion
transfer into a 15ml tube, suck out 3ml for transmission, and dilute the remaining 3ml to 6ml with pechil
add the diluted pge to a 24-well plate at 500 microns per hole, and then test luciferase

X.Molecular Colon basic protocols

1.PCR Reaction

Reagent	Volume(μl)
5X Buffer	10
DMSO	4
dNTP	4
Forward Primer	2
Reverse Primer	2
Targeted DNA fragment	1
phusion	1
ddH₂O	26
In Total	50

2.PCR production purification

——QIAquick^R PCR Purification Kit

PB Buffer was added to the PCR product at a volume of 5:1
The sample was added into the column, centrifuged for 30-60s, and the supernatant was discarded after centrifugation
Add 750 micron Buffer PE column, centrifuge for 30-60s and discard supernatant
Then centrifuge for 1min and discard the residual liquid
Insert the column into the ep tube
Add 50 micron PB Buffer(10m micron Tris*HCL,pH8.5) or HO(ph 7.0-8.5) to the center of the membrane and centrifuge for 1min.2Elution with 30 microns will increase the concentration and centrifuge after 1min

3.Gel recycling