Difference between revisions of "Part:BBa K4479012"

(LAMP on qPCR)
 
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==F3 LAMP Primer for Oak Wilt V4==
 
==F3 LAMP Primer for Oak Wilt V4==
  
Loop-mediated Isothermal Amplification is a cheap and quick method to amplify a desired DNA target. LAMP uses four to six primers; F3, B3, FIP (Forward Inner Primer),  BIP (Backward Inner Primer), and the optional LF (Loop Forward) and LB (Loop Backward) primers. We are using the four primer system that recognises six regions on our target DNA and they will form dumbbell-shaped amplicons. Our lamp primers run at 71°C and they are deactivated at 95°C. The primers were designed with the Primer Explorer software, then ranked for competency using a computer model. This is the F3 Primer of our first set of LAMP primers designed for the MCM7 region of Bretziella fagacearum (MG270170.1).
+
Loop-mediated Isothermal Amplification is a cheap and quick method to amplify a desired DNA target. LAMP uses four to six primers; F3, B3, FIP (Forward Inner Primer),  BIP (Backward Inner Primer), and the optional LF (Loop Forward) and LB (Loop Backward) primers. We are using the four primer system that recognises six regions on our target DNA and they will form dumbbell-shaped amplicons. Our lamp primers run at 71°C and they are deactivated at 95°C. The primers were designed with the GLAPD software, then ranked for competency using a computer model. This is the F3 Primer of our first set of LAMP primers designed for the MCM7 region of Bretziella fagacearum (MG270170.1).
  
 
https://static.igem.wiki/teams/4479/wiki/parts-images/lamp-mcm7-g2-dna.jpg
 
https://static.igem.wiki/teams/4479/wiki/parts-images/lamp-mcm7-g2-dna.jpg
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==Characterization==
 
==Characterization==
 
===LAMP on qPCR===
 
===LAMP on qPCR===
To show that the primer set is working and to verify the amount of time the assay requires to run, we conducted our LAMP test on a qPCR machine. A green fluorescent dye was added to the LAMP master mix for data collection. The total volume of each reaction is 25 uL. We also decided to run the assay with different concentrations of target DNA (10 uL, 5 uL, 1 uL, 0.5 uL, and 0.1 uL). The primers were mixed at a 7:7:2:2 ratio (F3:B3:FIP:BIP). The results showed that all the trials passed the threshold, meaning that amplification was a success. The average time for amplification can be seen in Table 1.
+
To show that the primer set is working and to verify the amount of time the assay requires to run, we conducted our LAMP test on a qPCR machine. A green fluorescent dye was added to the LAMP master mix for data collection. The total volume of each reaction is 25 uL. We also decided to run the assay with different concentrations of target DNA (10 uL, 5 uL, 1 uL, 0.5 uL, and 0.1 uL). The primers were mixed at a 7:7:2:2 ratio (F3:B3:FIP:BIP). The results showed that all the trials passed the threshold, meaning that amplification was a success.  
 
+
{| class="wikitable" style="float:right; margin-left: 10px; margin-right: 20px"
 +
|+ Time for Detection with Different Concentrations of Target DNA
 +
|-
 +
! Conc. (ng/uL) !! Time (min)
 +
|-
 +
! scope="row" | 10
 +
|33.65 ± 4.52
 +
|-
 +
! scope="row" | 5
 +
|32.97 ± 2.87
 +
|-
 +
! scope="row" | 1
 +
|32.78 ± 1.75
 +
|-
 +
! scope="row" | 0.5
 +
|35.66 ± 3.23
 +
|-
 +
! scope="row" | 0.1
 +
|32.45 ± 8.65
 +
|-
 +
! scope="row" | Average
 +
|34
 +
|}
 
https://static.igem.wiki/teams/4479/wiki/wetlab-results/glapd2-amp.png
 
https://static.igem.wiki/teams/4479/wiki/wetlab-results/glapd2-amp.png
  
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|+ Melting Temperature of Different Concentrations of Target DNA
 
|+ Melting Temperature of Different Concentrations of Target DNA
 
|-
 
|-
! Conc. (ng/uL) !! Temp (°C) ± STDEV
+
! Conc. (ng/uL) !! Temp (°C)
 
|-
 
|-
 
! scope="row" | 10
 
! scope="row" | 10

Latest revision as of 18:48, 13 October 2022

F3 LAMP Primer for Oak Wilt V4

Loop-mediated Isothermal Amplification is a cheap and quick method to amplify a desired DNA target. LAMP uses four to six primers; F3, B3, FIP (Forward Inner Primer), BIP (Backward Inner Primer), and the optional LF (Loop Forward) and LB (Loop Backward) primers. We are using the four primer system that recognises six regions on our target DNA and they will form dumbbell-shaped amplicons. Our lamp primers run at 71°C and they are deactivated at 95°C. The primers were designed with the GLAPD software, then ranked for competency using a computer model. This is the F3 Primer of our first set of LAMP primers designed for the MCM7 region of Bretziella fagacearum (MG270170.1).

lamp-mcm7-g2-dna.jpg

Characterization

LAMP on qPCR

To show that the primer set is working and to verify the amount of time the assay requires to run, we conducted our LAMP test on a qPCR machine. A green fluorescent dye was added to the LAMP master mix for data collection. The total volume of each reaction is 25 uL. We also decided to run the assay with different concentrations of target DNA (10 uL, 5 uL, 1 uL, 0.5 uL, and 0.1 uL). The primers were mixed at a 7:7:2:2 ratio (F3:B3:FIP:BIP). The results showed that all the trials passed the threshold, meaning that amplification was a success.

Time for Detection with Different Concentrations of Target DNA
Conc. (ng/uL) Time (min)
10 33.65 ± 4.52
5 32.97 ± 2.87
1 32.78 ± 1.75
0.5 35.66 ± 3.23
0.1 32.45 ± 8.65
Average 34

glapd2-amp.png

To verify if the amplification was on target, we looked at the melting curve from the qPCR machine. There is only 1 peak and they are within the acceptable deviation range, so we conclude that the primer set is able to amplify the target gene successfully.

Melting Temperature of Different Concentrations of Target DNA
Conc. (ng/uL) Temp (°C)
10 86.35 ± 0.11
5 85.94 ± 0.47
1 86.06 ± 0.45
0.5 86.46 ± 0.39
0.1 86.49 ± 0.63
Average 86.26

glapd2-melt.png