Reagent List for the Experiment
|
Category |
Cat.No. |
Product name |
|
DNA Library Preparation |
12972ES |
|
|
Magnetic Beads |
12601ES |
Hieff NGSTM DNA selection Beads (Superior Ampure XP alternative) |
|
Quantification |
12642ES |
|
|
Adapters |
13352ES |
|
|
User-Supplied Materials |
— |
Absolute Ethanol |
Pre-Experiment Preparation
1. Equilibrate magnetic beads to room temperature before use.
2. Prepare 80% ethanol.
3. Dilute the adapters 2-fold.
4. Prepare the samples according to the volumes specified in the table below.
|
Sample ID |
1 |
2 |
3 |
4 |
5 |
6 |
|
Species / Tissue |
Wheat Leaf |
Rice Leaf |
Rice Seed |
Soybean Seed |
Corn Seed |
Sugarcane Leaf |
Product description
|
Library Preparation Method |
Manual library preparation(Enzymatic fragmentation) |
|
Input DNA |
200 ng |
|
Fragmentation |
4℃ 1 min,30℃ 15 min,72℃ 20 min,4℃ hold |
|
Adapter |
MGI UDI adapter, 2-fold dilution |
|
Post-Ligation Cleanup & Size Selection |
0.8× purification after ligation |
|
Post-Ligation Cleanup & Size Selection |
Size selection 0.6×/0.2× |
|
PCR Cycles |
7 cycles |
|
Post-PCR Cleanup |
0.9× purification |
|
Library Elution Volume |
40 μL |
Procedure
1. DNA Fragmentation / End Repair / dA-Tailing
After thawing the reagents listed in Table 1, vortex to mix, and place on ice for later use. Prepare the reaction mixture (as shown in Table 1) on ice. Mix gently by pipetting or vortexing at low speed, then perform a quick pulse centrifugation to collect the reaction solution at the bottom of the tube. Incubate according to the reaction program in the table to perform DNA fragmentation, end repair, and dA-tailing reactions.
Table 1. PCR Reaction for DNA Fragmentation / End Repair / dA-Tailing
|
Reaction System |
Reaction Program |
||
|
Reaction Component |
Volume (μL) |
Temperature |
Time |
|
Input DNA |
200 ng |
Heated Lid: 105 °C |
On |
|
SmearaseTM Buffer 4.0 |
10 |
4℃ |
1 min |
|
SmearaseTM Enzyme 4.0 |
10 |
30℃ |
15 min |
|
ddH2O |
Up to 60 |
72℃ |
20 min |
|
- |
- |
4℃ |
Hold |
2. Adapter Ligation
The Adapter concentration must be diluted according to the Input DNA amount. For this experiment, the UDI adapters are diluted 2-fold.
After thawing the reagents listed in Table 2, vortex to mix and place on ice for later use. Prepare the reaction mixture (as shown in Table 1) on ice. Mix gently by pipetting or vortexing, then perform a quick pulse centrifugation to collect the reaction solution at the bottom of the tube. Incubate according to the program in Table 2 to perform the adapter ligation reaction.
Table 2. Adapter Ligation Reaction
|
Name |
Volume (μL) |
Temperature |
Time |
|
dA-tailed DNA |
60 |
- |
- |
|
Ligation Enhancer 4.0 |
30* |
Heated Lid |
Off |
|
Rapid DNA Ligase 4.0 |
10 |
20℃ |
15 min |
|
UDB Adapter |
5 |
4℃ |
Hold |
|
ddH2O |
Up to 110 |
- |
- |
【Note】:* Ligation Enhancer is viscous. Before use, invert and vortex thoroughly to mix completely, then briefly centrifuge.
3. Post Ligation Clean Up
This step uses magnetic beads to purify adapter-ligated products, removing unligated adapters and adapter dimers.
A “purify-then-size-select” strategy was used: first, 0.8× cleanup followed by elution in 102 μL ddH₂O; then, double-sided size selection at 0.6×/0.2×. The final product was eluted in 20 μL for downstream amplification.
4. Library Amplification
This step performs PCR amplification to enrich the purified and size-selected adapter-ligated products. Prepare the reaction mixture and set the cycling program according to Table 3.
Table 3. Library Amplification Reaction
|
Name |
Volume (μL) |
Temperature |
Time |
Cycle Numbe |
|
Adapter Ligated DNA |
20 |
98℃ |
45 sec |
1 |
|
2×Ultima HF Amplification Mix |
25 |
98℃ |
|
7 |
|
Primer Mix(12330ES) |
5* |
60℃ |
30 sec |
|
|
Total |
50 |
72℃ |
30 sec |
|
|
- |
- |
72℃ |
1 min |
1 |
|
- |
- |
4℃ |
Hold |
- |
5. Magnetic Bead Purification of Amplified Products
The amplified products were purified using Hieff NGSTM DNA Selection Beads(0.9×,Beads:DNA=0.9:1)
6. Library Quality Control
|
Sample ID |
1 |
2 |
3 |
4 |
5 |
6 |
|
Sample |
Wheat Leaf |
Rice Leaf |
Rice Seed |
Soybean Seed |
Corn Seed |
Sugarcane Leaf |
|
Elution Conc. (ng/μL) |
56.6 |
64.6 |
55.2 |
48.4 |
39.8 |
37.4 |
|
Library Yield (ng) |
2264 |
2584 |
2208 |
1936 |
1592 |
1496 |
Agarose Gel Electrophoresis of the Libraries (The brightest band of the Marker indicates 500 bp)
Analysis of Experimental Results
Plant breeding samples (rice, wheat, soybean, corn, and sugarcane) were processed using the enzyme-based library preparation kit 12972ES. The resulting libraries exhibited high yields, tight fragment size distributions, and met the quality control standards.