Notebook | HWFLA-Beijing

2024.8.19

Participants

Li Jialiang, Wu Siyuan, Liu Lanxin, Li Tianyi

Goal

Prepare LB medium (1L) for bacterial culture
Prepare 100mg/ml Ampicillin
Prepare 0.05mol/L CaCl2
Inoculate Azurin template strain, anti-PD-L1 template strain, plactate1 template strain, plactate2 template strain

Content

1.Prepare LB medium (1L) for bacterial culture

LB liquid:

Material	Dosage
Yeast extract	5g
Trypsin	10g
Sodium chloride	10g

LB Solid

Material	Dosage
LB liquid	100ml
Agar powder	1.5g

Sterilize at high temperature 121℃, 15min

Prepare a 10ml Ampicilin solution with a final concentration of 100μg/mL

Prepare 0.05mol/L CaCl2

Material	Dosage
CaCl2	0.28g
Water	100ml

Mix and sterilise at high temperature121℃，15min

Prepare 0.05mol/L CaCl2 with glycerin

Material	Dosage
CaCl2	0.28g
15% glycerin	15ml
Water	100ml

Mix and sterilize at high temperature121℃, 15min

Inoculate 4 kinds of template bacteria solution

Promoter template	Target gene template
Plactate1 (LldR)	Azurin
Plactate2 (LldR-new)	anti-PD-L1

Get four combinations using them：Plactate1-Azurin、Plactate1-anti-PD-L1、Plactate2-Azurin、Plactate2-anti-PD-L1
Using a benchtop to inoculate 5ml of LB、5μL of Ampicilinand 50ul of bacteria solution

2024.8.20

Participants

Li Jialiang, Wu Siyuan, Liu Lanxin, Li Tianyi

Goal

Plasmid extraction
PCR amplification
Use agarose gel electrophoresis to detect whether DNA was obtained
DNA recovery

Content

Plasmid was extracted：

Material	Dosage
Solution I: SP1 bacterial suspension	250μL
Solution II: SP2 cell lysis buffer	250μL
Solution III: SP3 neutralization solution	350μL
Wash solution	750μL

1-5ml of bacterial culture (P1, P2, Azurin, anti-PD-L1) was centrifuged at 12000rpm for 1min, and the supernatant was absorbed

Add 250μL solution to the centrifugation tube containing the bacterial precipitation and suspend the bacterial cell precipitation thoroughly using a vortex oscillator
Add 250μL solution Ⅱ into the centrifuge tube and gently turn it up and down 6-8 times to fully crack the bacteria. At this time, the bacteria solution will become clear and viscous
Add 350u solution III into the centrifuge tube and turn it up 6-8 times to mix well. The white, fluffy precipitate will appear at this time. Centrifuge at 12000rpm for 10min and transfer the supernatant to another clean centrifuge tube
Add 0.35 times the volume of anhydrous ethanol and mix well
Add the supernatant into the adsorption column, leave at room temperature for 2min, centrifuge at 12000rpm for 1min, drain the waste liquid in the collection tube, and put the adsorption column back into the collection tube
Add 750μL bleach solution to the adsorption column, centrifuge at 12000rpm for 1min, and put the adsorption column into the collection tube
Add 700L bleaching solution to the adsorption column, centrifuge at 12000rpm for 1min, and put the adsorption column into the collection tube
Centrifuge at 12000rpm for 2min and place the adsorption column at room temperature or 50℃ for several minutes
Place the adsorption column into a clean centrifuge tube, drop 50μL eluent preheated in a water bath at 65℃ into the center of the adsorption film, place at room temperature for 2min, and centrifuge at 12000rpm for 1min
The eluent obtained was re-added into the adsorption column, placed at room temperature for 2min, and centrifuged at 12000rpm for 1min

PCR amplification (target gene amplification)：

Material	Dosage
Target gene (P1, P2, anti-PD-L1, Azurin)	2 μL
2*Mix (dNTP, DNA polymerase, Buffer, magnesium ion)	25 μL
Primer (F)	2 μL
Primer (R)	2 μL
ddH2O	19 μL

Set up the PCR reaction program
Set up the PCR reaction program

1.Pre degeneration： Double chain to single chain 95°C，5min

2.dimorphism:95°C，30s

3.annealing：55°C，30s （Repeat 1-3 30 times）

4. extending：72°C，30s for gene /2min for plasmid

5. 72 ℃，10 min

6. 4°C，∞

Initiate the program
Agarose gel electrophoresis was used to detect whether DNA was amplified
Prepare50mL agarose gel

Material	Dosage
Agarose powder	0.5 g
TAE buffer solution	50 mL
Nucleic acid dye	3 μL

Melt agarose powder and TAE buffer at high temperature and add 3μL nucleic acid dye
Install the electrophoresis tank
Gently pour the electrophoresis solution cooled to 60 °C onto the horizontal plate of the electrophoresis tank
After it has solidified, add the electrophoresis buffer to the bath and pull out the comb
Add the mixture to the sample tank
Connect one end of the sample hole to the negative electrode and the other to the positive electrode. Turn on the power supply, adjust the voltage to 180V, and electrophoresis for 20min
The gel was removed and observed under an ultraviolet lamp. The DNA bands with red fluorescence were found

DNA gel extraction

Material	Dosage
Glue solution	300 μL / 0.1 g DNA gel block
Bleach wash solution	600 μL

After agar-gel electrophoresis, a single DNA strip of interest is cut from the agar-gel and weighed
Add 600μL sol solution to the glue block and place in a water bath at 55℃ for 10 min. During the process, gently turn the centrifuge tube up and down continuously to ensure that the glue block is fully dissolved
The solution was added to an adsorption column and centrifuged at 12000pm for 60 seconds
Add 600μL bleaching solution to the adsorption column and centrifuge at 12000rpm for 1min, discard the waste liquid, and put the adsorption column into the collection tube
Add 600μL bleach solution into the adsorption column, centrifuge 12000rpm for 1min, discard the waste liquid, and put the adsorption column into the collection tube
Centrifuge at 12000rpm for 2min, remove the bleach solution as much as possible, and place the adsorption column open at room temperature or 50℃ in a temperature box
Place the adsorption column into a clean centrifuge tube, drop the appropriate amount of eluent preheated in a water bath at 65℃ into the center of the adsorption film, place at room temperature for 2min, and centrifuge at 12000rpm for l min
DNA products stored at -20℃

Result

A. plactate1, plactate2 plasmid skeleton amplification, the size are 3150bp and 3800bp
plactate1-Azurin, plactate2-Azurin, plactate1-anti-PD-L1, plactate2-anti-PD-L1, target gene amplification size is 550bp

2024.8.21

Participants

Li Jialiang, Wu Siyuan, Liu Lanxin, Li Tianyi, Wu Peiran

Goal

The target gene sfGFP was obtained by PCR
Recombinant plasmid was constructed by homologous recombination
The recombinant product transformed Escherichia coli BL21

Content

The target gene sfGFP was obtained by PCR
PCR system
Target gene (P1, P2, sfGFP): 2μL
2*Mix (dNTP, DNA polymerase, Buffer, magnesium ion): 25 uL
Primer (F/R): F:2μL R:2μL
ddH2O: 19μL set the PCR reaction program
Procedure: Pre degeneration: double chain to single chain 95°C，5min
Degeneration：95°C，30s
Annealing：55°C，30s （Repeat 30 times）
Extending：72°C，30s for GFP /2min for plasmid
72 ℃，10 min
4°C，∞
agarose gel formula

Material	Dosage
Total	50 mL
Agarose	0.5 g
1*TAE	50 mL

After 2 minutes of high-fire melting, add 3μL of dye and pour it into the mold.

Homologous recombination
the amount of DNA required for the recombination reaction was calculated according to the formula, and the amount of each component added was not less than 1μl
Prepare the following reaction system on the ice:

Component	Recombination reaction
Linearized carrier	2 μL
Target gene segment	1 μL
2 × ClonExpress Mix	5 μL
ddH2O	2 μL

Use a pipette to gently suck and mix (do not shake and mix), and briefly centrifuge to collect the reaction liquid to the bottom of the tube. 50℃, 15 min; Reduce to 4 ° C or cool immediately on ice

Transformation of recombinant products
Thawing chemoreceptor cells for cloning on ice
Add 10 μl recombinant product into 100 μL receptive cells, gently mix the tube wall (do not shake and mix), and leave it on ice for 30 min.
After the 42℃ water bath is heated for 45 seconds, it is immediately placed on ice to cool for 3 min.
Add 900 μL LB liquid medium (without antibiotics) and shake the bacteria at 37℃ for 1 h (rotational speed 200 rpm).
Preheat the corresponding resistant LB solid medium plate in a 37℃ incubator.
Centrifuge at 5000 rpm (2,500 × g) for 5 min and discard 900 μL supernatant. The bacteria sediment was suspended with the remaining medium and lightly coated with a sterile coating stick on a plate containing Amp resistance.
Culture inversely in an incubator at 37℃ for 12 h.

Result

Left：plactate1, placate2 Plasmid skeleton amplification size are 3150bp and 3800bp
Right：plactate1-sfGFP, plactate2-sfGFP amplification size are both 750bp

2024.8.22

Participants

Li Jialiang, Wu Siyuan, Liu Lanxin, Li Tianyi

Goal

Colony PCR verification
Inoculate the correct single colony

Content

PCR amplification (colony expansion):
The target genes anti-PD-L1, Azurin, and sfGFP were amplified by PCR
Material dose
DNA Template: 6 recombinant plasmid colonies (anti-PD-L1, Azurin, GFP)
2*Mix (dNTP, DNA polymerase, Buffer, magnesium ion) 10μL
(F/R): F:1μL R:1μL
ddH2O: 8μL
Set up the PCR reaction program
- Predegeneration: double chain to single chain95°C，5min
- degeneration：95°C，30s
- Annealing：55°C，30s
- Extending：72 °C，1min Step 2-4 repeat 30 times
- 72°C, 10 min
- 6. 4°C, ∞
Prepare50mL agarose gel
Material dose
Agarose powder 1g
TAE buffer 100mL
Nucleic acid dye 18μL
Melt agarose powder and TAE buffer at high temperature and add 6μL nucleic acid dye
* Install the electrophoresis tank
* Gently pour the electrophoresis solution cooled to 60°C onto the horizontal plate of the electrophoresis tank
* After it solidifies, add the electrophoresis buffer to the electrophoresis tank and then pull out the comb
* Add the mixture to the sample tank
* One end of the electrophoresis point sample hole is connected to the negative electrode, and the other end is connected to the positive electrode; turn on the power supply,
* Adjust voltage to 180V, electrophoresis 20min
* Remove the gel and observe it under an ultraviolet lamp. The red fluorescent bands are DNA bands
Verify the correct colony by inoculation
plactate1-Azurin, plactate2-Azurin, plactate1-anti-PD-L1, plactate2-anti-PD-L1
4mL LB solution + correct colony +4uL Ampicilin was cultured at 37 ° C for 12h

Result

plactate1-sfGFP, plactate2-sfGFP, Recombinant plasmid validation
A: Colony PCR validation diagram
B: Plate colony map
C: Sequencing diagram

plactate1-Azurin, plactate2-Azurin, plactate1-anti-PD-L1, plactate2-anti-PD-L1
Recombinant plasmid validation
A: Colony PCR validation diagram
B: Plate colony map
C: Sequencing diagram

2024.8.23

Participants

Li Jialiang, Wu Siyuan, Liu Lanxin, Li Tianyi, Wu Peiran

Goal

Plasmid extraction (plactate1-Azurin, plactate1-anti-PD-L1, plactate2-Azurin, plactate2-anti-PD-L1)
Inoculate ECN 1917 to make ECN 1917 receptive state
Heat shock transformation of recombinant plasmid to ECN 1917
Expanded culture of Plactae1-GFP and Plactate2-GFP with different lactic acid-induced expression (cultured at 18℃ for 20h)

Content

Plasmid extraction (same steps as 2024.8.20)
Inoculate ECN 1917 to make ECN 1917 receptive state
- Transfer ECN1917 bacteria solution cultured overnight at 1% inoculation rate (37℃, 220rpm, culture for 2.5h to 0.3 for OD600)
- bacterial harvest: Centrifuge at 4℃ 5000rpm for 5 min after ice bath
- Wash precipitate in cold deionized water and centrifuge at 4°C5000rpm for 5 min
- precipitation Add 2ml of 0.05mol/l CaCl2-15% glycerol mixture to cold, gently blow away, and take an ice bath of 0.05mol/l CACL2-
- 15% glycerol mixture for 5 minutes
- The receptive cell suspension was formed by adding 2ml of cold 0.05mol/l CaCl2-15% glycerol mixture and gently blowing it away. Divided into 50-100μL small parts, stored at -70℃
Heat shock conversion (same steps as 2024.8.21)
plactate1-sfGFP and plactate2-sfGFP were cultured with different concentrations of lactic acid (0mM, 2mM, 5mM, 10mM) to induce the expression of GFP fluorescent protein

Result

Converted to ECN 1917
A: Colony PCR validation diagram in ECN1917
B: Plate colony map

2024.8.24

Participants

Wu Siyuan, Liu Lanxin, Li Tianyi, Wu Peiran

Goal

Colony PCR verified whether the recombinant plasmid was transformed into EcN 1917
Inoculate the correct single colony
The expression of fluorescent protein sfGFP was detected

Content

PCR amplification (colony amplification) :
PCR amplification of target genes P1, P2, anti-PD-LI, Azurin in EcN(550bp)
Material dose
1 colony (P1, P2, anti-PD-L1, Azurin, GFP)
2*Mix (dNTP, DNA polymerase, Buffer, magnesium ion) 10μL
(F/R) : F:1μL R:1μL
ddH2O 8μL
• Set up PCR reaction procedures
1. Predenaturation: double chain to single chain 95°C, 5min
2.Denaturation: 95°C, 30s
3. Annealing: 55°C, 30s
4. Extension: 72 °C, 30s
2-4 Repeat 30 times 5. 72°C, 10 min
6. 4°C, ∞
Configure 100mL agarose gel
Material dose
Agarose powder 1g
TAE buffer 100mL
Nucleic acid dye 6μL
Melt agarose powder and TAE buffer at high temperature and add 6μL nucleic acid dye
* Install the electrophoresis tank
* Gently pour the electrophoresis solution cooled to 60°C onto the horizontal plate of the electrophoresis tank
* After it has solidified, add the electrophoresis buffer to the electrophoresis tank and then pull out
Comb
* Add the mixture to the sample tank
* One end of the electrophoresis point sample hole is connected to the negative electrode, the other end is connected to the positive electrode; turn on the power supply,
* Adjust voltage to 180V, electrophoresis 20min
*Remove the gel and observe it under an ultraviolet lamp. The red fluorescent bands are DNA bands
GFP fluorescence determination
- Fluorescence microscope detection, sfGFP luminescence.
- ELISA reading (black 96-well plate, 470nm excitation light, 509nm emission light, reading value; Transparent 96-well plate, OD600 reading value; Former reading/latter reading = relative fluorescence intensity)
Verify the correct colony by inoculation
plactate1-Azurin, plactate2-Azurin, plactate1-anti-PD-L1, plactate2-anti-PD-L1 in EcN
4mL LB solution + correct colony +4μL Amp+ was cultured at 37 ° C for 12h

The luminescence of sfGFP was observed by a fluorescence microscope.

2024.8.25

Participants

Li Jialiang, Wu Siyuan, Liu Lanxin, Li Tianyi, Wu Peiran

Goal

The 4 EcN strains successfully transformed by expanded culture were cultured at 37 degrees for 2-4h.
Set different culture OD and other lactic acid induction concentrations and induce culture at 37 degrees for more than 10h
Configure different concentrations of lactic acid, 0mM, 2mM, 5mM, 10mM

Content

The 4 EcN strains successfully transformed by expanded culture were cultured at 37 degrees for 2-4h.
The correct 4 plasmids were transformed into Escherichia coli ECN, the correct clone and the correct clone, and the correct clone was inoculated into seed liquid.
Then, the seed solution was transferred to amplify E.coli until OD=0.5-0.6.
Set different culture OD and other lactic acid induction concentrations and induce culture at 37℃ for more than 10h
Lactic acid was added for induction (the final concentration was 0 25 10mM), the bacterial solution and supernatant were collected for about 10 hours (the ECN clone was selected to culture overnight, and the ratio of 1 to 100 was inoculated into the medium containing lactic acid), and the protein expression was subsequently detected.

Result

2024.8.27

Participants

Li Jialiang, Wu Siyuan, Liu Lanxin, Li Tianyi, Wu Peiran

Goal

Culture four strains to induce expression
Broke the protein
Make SDS-PAGE protein measuring gel

Content

Cultivate Four Strains and Induce Expression
To induce the expression of four proteins, we used 0mM, 2mM, 5mM, and 10mM lactic acid, respectively. Obtain the bacterial suspensions cultured overnight and centrifuge them at 4°C, 5000rpm, for 5 minutes to separate the supernatant from the precipitate. Discard the supernatant and retain the precipitate. Resuspend the residue in 10 ml of PBS buffer. Repeat the centrifugation process at 4°C, 5000rpm for 5 minutes, discard the supernatant, retain the residue, and resuspend it in 10ml of PBS buffer.
Protein Disruption
Perform ultrasonic disruption at 100w with a 3-second on and 3-second off cycle for 10 minutes. Ensure the entire process is conducted on ice, with 16 sets. After disruption, centrifuge to collect the supernatant, discard the residue, and measure the protein concentration.
Preparation of SDS-PAGE Gel for Protein Analysis
Assemble the required equipment and apparatus. Then, prepare the upper stacking and lower resolving gel using a 10% PAGE gel solution.

2024.8.28

Participants

Li Jialiang, Wu Siyuan, Liu Lanxin, Li Tianyi, Wu Peiran

Goal

Prepare protein sample
Test the expression of protein

Content

Prepare protein sample
The bacterial supernatant was added to 5xSDS-PAGE protein loading buffer and thoroughly mixed. Heat the mixture at 100℃ for10min, then 12000rpm centrifuge for 2min. The supernatant was subjected to electrophoresis by 10%SDS-PAGE.
Test the expression of protein
It is necessary to ensure that the protein content of the samples is consistent and that the size of target proteins in the electrophoresis results are consistent through Coomassie bright blue staining.

2024.8.29-9.15

Participants

Li Jialiang, Wu Siyuan, Liu Lanxin, Li Tianyi, Wu Peiran

Goal

Write experimental data processing and wiki writing

Content

Complete the experimental data processing and wiki.