Reagent List for the Experiment
|
Category |
Cat.No. |
Product name |
|
DNA Library Preparation |
12340ES |
|
|
mRNA Isolation |
12629ES |
|
|
Magnetic Beads |
12601ES |
Hieff NGSTM DNA selection Beads (Superior Ampure XP alternative) |
|
Quantification |
12642ES |
|
|
Adapters |
12330ES |
|
|
User-Supplied Materials |
— |
Absolute Ethanol |
|
Control Reagent |
— |
NEB ultra II directional kit with Poly A selection |
Pre-Experiment Preparation
1. Equilibrate magnetic beads to room temperature before use.
2. Prepare 80% ethanol.
3. Sample Preparation: human(pure T cells or mixed cells), mouse(brain), plant(wheat, Stem internode)
Product description
|
Library Preparation Method |
mRNA library preparation |
|
Input RNA |
200 ng, 500 ng |
|
Fragmentation |
94 °C for 7 min |
|
Adapter |
Illumina UDI adapter, 3 μM-5 μL |
|
Post-Ligation Cleanup & Size Selection |
0.6× cleanup after ligation; double-sided size selection at 0.6× / 0.2× |
|
PCR Cycles |
14 cycles, 12 cycle |
|
Post-PCR Cleanup |
0.9× purification |
|
Library Elution Volume |
30 μL |
Procedure
1. mRNA Purification and Fragmentation
This protocol describes the enrichment of poly(A)+ mRNA from high-quality eukaryotic total RNA (Animals, Plants, Fungi) using Hieff NGSTM mRNA Isolation Master Kit V2 (Yeasen Cat#12629).
- Input Material: 10 ng – 4 μg Total RNA (RIN > 7). In this experiment, Input RNA 200 ng, 500 ng.
- Volume: Adjust RNA volume to ≤50 μL with Nuclease-Free Water.
- Note: Not suitable for FFPE samples or RNA lacking poly(A) tails.
1. Bind mRNA
Equilibrate beads to room temperature (~30 min).
Mix 50 μL Total RNA (10 ng–4 μg) + 50 μL Beads. Pipette 6×.
Incubate (Thermal Cycler): 65°C for 5 min, 25°C for 5 min, Hold at 25°C
2. Wash & Elute
Separate on magnet (5 min). Discard supernatant.
Wash with 200 μL Wash Buffer. Pipette 6×. Separate on magnet. Discard supernatant.
Repeat wash step once (Total 2 washes).
Elute by resuspending in 50 μL Tris Buffer. Pipette 6×.
Incubate (Thermal Cycler): 80°C for 2 min, Hold at 25°C
3. Re-bind
Add 50 μL Binding Buffer. Pipette 6×. Incubate at Room Temperature for 5 min.
Separate on magnet (5 min). Discard supernatant.
Wash with 200 μL Wash Buffer. Pipette 6×. Separate on magnet. Discard supernatant completely.
4. Fragment
Resuspend beads in 18.5 μL Frag/Prime Buffer. Pipette 6×.
Incubate in Thermal Cycler (Pre-heated to 94°C) based on desired size. In this experiment, the RNA was fragmented at 94°C for 7 minutes.
Table 1. Recommended mRNA Fragmentation Procedure
|
Target Insert Size (bp) |
Fragment condition |
|
200-300 |
94℃, 10 min, 4℃, hold; |
|
300-400 |
94℃, 7 min, 4℃, hold; |
|
400-500 |
94℃, 5 min, 4℃, hold; |
Separate immediately on magnet. Transfer 17 μL supernatant to a new tube.
Proceed to First-Strand cDNA Synthesis.
2. 1st cDNA Strand Synthesis
This step synthesizes first-strand cDNA from enriched/fragmented target RNA (prepared via Poly(A) selection or rRNA depletion).
Reagent Preparation: Thaw the 1st strand synthesis reagents on ice, mix well by pipetting.
Reaction Setup: Assemble the reaction mixture in a PCR tube and perform the cDNA synthesis reaction.
Table 2. cDNA synthesis reaction system and Procedure
|
Reaction System |
Reaction Program |
||
|
Reaction Component |
Volume (μL) |
Temperature |
Time |
|
Frag/Prime Buffer with Fragmented RNA |
17 |
Heated Lid: 105 ℃ |
On |
|
25℃ |
10 min |
||
|
1st Reaction Module 2.0 |
8 |
42℃ |
15 min |
|
Total |
25 |
70℃ |
15 min |
|
- |
- |
4℃ |
Hold |
3. 2nd cDNA Fragmentation / End Repair / dA-Tailing
Thaw all reagents listed in Table 1, invert to mix thoroughly, and keep on ice. On ice, prepare the reaction mixture as specified in Table 1. Gently pipette up and down or use low-speed vortexing to mix, then briefly centrifuge to collect the reaction liquid at the bottom of the tube.
Table 3. PCR Reaction for DNA Fragmentation / End Repair / dA-Tailing
|
Reaction System |
Reaction Program |
||
|
Reaction Component |
Volume (μL) |
Temperature |
Time |
|
1st Strand cDNA |
25 |
Heated Lid: 105 ℃ |
On |
|
2nd Reaction Module (dUTP)* |
35 |
16℃ |
30 min |
|
Total |
60 |
72℃ |
15 min |
|
- |
- |
4℃ |
Hold |
4. Adapter Ligation
The adapter should be diluted to an appropriate concentration based on the input DNA amount. Thaw all reagents listed in Table 4, invert to mix thoroughly, and keep on ice. On ice, prepare the reaction mixture as specified in Table 4. Perform the adapter ligation reaction according to the program in Table 4.
Table 4. Adapter Ligation Reaction
|
Name |
Volume (μL) |
Temperature |
Time |
|
dA-tailed DNA |
60 |
Heated Lid |
Off |
|
Ligation Reaction Module |
35 |
20℃ |
15 min |
|
PE Adapter |
5*(3 μM) |
4℃ |
Hold |
|
ddH2O |
Up to 100 |
- |
- |
【Note】:* Ligation Enhancer is viscous. Before use, invert and vortex thoroughly to mix completely, then briefly centrifuge.
5. Post Ligation Clean Up
This step uses magnetic beads to purify the adapter-ligated products. Purification removes unligated adapters or adapter dimers and other ineffective byproducts.
In this experiment, a post-ligation cleanup followed by size selection was used: perform 0.6× cleanup on the ligation product, elute with 102 μL ddH2O, then carry out size selection at a ratio of 0.6×/0.2×. The final product was eluted in 20 μL for the next amplification step.
6. 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℃ |
1 min |
1 |
|
2×Super CanaceTM II High-Fidelity Mix |
25 |
98℃ |
10 sec |
11~16 |
|
Primer Mix(12330ES) |
5* |
60℃ |
30 sec |
|
|
Total |
50 |
72℃ |
30 sec |
|
|
- |
- |
72℃ |
5 min |
1 |
|
- |
- |
4℃ |
Hold |
- |
7. Magnetic Bead Purification of Amplified Products
The amplified products were purified using Hieff NGSTM DNA Selection Beads (0.9×, Beads:DNA = 0.9:1).
8. Library Quality Control
|
Kit → |
Yeasen 12629+12340 |
NEB |
|||
|
Library Conc.(ng/μL) |
Library Conc.(nM, qPCR method) |
Library Conc.(ng/μL) |
Library Conc.(nM, qPCR method) |
||
|
Human |
200 ng |
38.4 |
179.75 nM |
2.6 ng/μL |
11.72 nM |
|
500 ng |
92.8 ng/μL |
453.98 nM |
7.04 ng/μL |
31.29 nM |
|
|
Mouse |
200 ng |
60.6 ng/μL |
350.91 nM |
5.56 ng/μL |
25.49 nM |
|
500 ng |
120 ng/μL |
639.97 nM |
8.52 ng/μL |
37.61 nM |
|
|
Wheat |
200 ng |
16.2 ng/μL |
75.07 nM |
0.85 ng/μL |
2.9 nM |
|
500 ng |
38.2 ng/μL |
180.91 nM |
2.9 ng/μL |
15.1 nM |
|
RNA-seq Insert Size Analysis
Gene Body Coverage Analysis
Strand Specificity Analysis
Analysis of Experimental Results
1. Library Yield
Yeasen demonstrated superior performance in library yield, with both Qubit (ng/μL) and qPCR (nM) quantification results being significantly higher than those of the NEB kit.
2. Insert Size
Both kits produced comparable insert sizes, with a distribution centered around 250-300 bp.
3. Gene Body Coverage
Yeasen Kit: Showed superior coverage at the 5' end of the transcripts.
NEB Kit: Exhibited stronger coverage intensity at the 3' end.
4. Strandedness
The Yeasen kit demonstrated better strand specificity than the NEB kit at both input amounts tested (200 ng and 500 ng).