Protocol for Transfection of mRNA into Cells

1. Experimental Materials

  • HEK 293 cell: Cell confluency should reach 70%–90%.
  • mRNA: EGFP mRNA, 1000 bp (Concentration ≥ 100 ng/μL)
  • Hieff TransTM Booster DNA&RNA Transfection Reagent (Cat#40801)
  • Serum-free Opti-MEM® (Reduced Serum Medium)
  • Compatible tissue culture plates and related lab consumables (using a 6-well plate as an example)

2. Experimental Procedure

1)Preparation One Day Before Transfection

  • Seed HEK293 cells in a 6-well plate at a density that will reach 70–90% confluency on the day of transfection.
  • Use 2 mL complete DMEM (with 10% FBS) per well.
  • Incubate at 37 °C, 5% CO₂ overnight

2)Prepare mRNA–Reagent Complex(per well of a 6-well plate)

  • Dilute mRNA: Dilute 2.5 μg EGFP mRNA in 100 μL Opti-MEM.

[Note]: mRNA concentration should be > 0.1  μg/μL to ensure accurate pipetting.

  • Dilute Transfection Reagent: In a separate tube, dilute 5 μL transfection reagent in 100 μL Opti-MEM.
  • Form mRNA-Transfection Reagent Complex: Combine the two solutions, mix gently, and incubate for 10–15 minutes at room temperature.

Plate Format

mRNA Amount per Well

Transfection Reagent Volume

Total Complex Volume (in Opti-MEM or serum-free medium)

6-well plate

2–3 μg

4–6  μL

200  μL

24-well plate

500–800 ng

1.5–2  μL

50  μL

96-well plate

100–200  ng

0.3–0.5  μL

20  μL

3)Cell Transfection: Add to Cells

  • Remove old culture medium from the well and replace with 1.8 mL fresh complete DMEM.
  • Add the 200 μL mRNA–reagent complex dropwise to the well.
  • Gently rock the plate to distribute evenly.

4)Post-Transfection Handling

  • Incubate cells at 37 °C, 5% CO₂.
  • Observe EGFP expression at 18–24 hours post-transfection using fluorescence microscopy.
  • No media change is needed unless cytotoxicity is observed.

Tips & Notes

  • Ensure mRNA is of high purity (DNase-treated, A260/A280 ~2.0).
  • Avoid repeated freeze-thaw cycles of mRNA stock.
  • This protocol can be adapted for other plate formats (e.g., 24-well or 96-well) by scaling volumes accordingly.

3. Experimental Result

1)Efficient mRNA Delivery in HEK293 cell

Figure 1. Transfection of 2.5 μg EGFP mRNA (~1000 bp) with 5 μL transfection reagent in a 6-well plate, showing high transfection efficiency. 

Figure 1. Transfection of 2.5 μg EGFP mRNA (~1000 bp) with 5 μL transfection reagent in a 6-well plate, showing high transfection efficiency.

2)Efficient mRNA Delivery in a Wide Range of Cell Types

Figure 2. mRNA Transfection Performance in Multiple Cell Lines

 Figure 2. mRNA Transfection Performance in Multiple Cell Lines

mRNA transfection across different cells using Booster DNA&RNA Transfection Reagent versus T brand L*3000. The result demonstrates superior mRNA transfection efficiency of Booster.

4. Customer Feedback

1) High-Efficiency 293T mRNA Transfection

Figure 3. mRNA Transfection Performance 

Figure 3. mRNA Transfection Performance 

2) High-Efficiency HTC116 mRNA Transfection

Figure 4. mRNA transfection using Booster DNA&RNA Transfection Reagent versus T brand L*3000. The result demonstrates superior mRNA transfection efficiency of Booster.

Figure 4. mRNA transfection using Booster DNA&RNA Transfection Reagent versus T brand L*3000. The result demonstrates superior mRNA transfection efficiency of Booster.

4. Frequently Asked Questions (FAQs) & Solutions

Q1: What is the optimal confluency for mRNA transfection?

A: Cells should be 70%–90% confluent at the time of transfection to ensure optimal uptake and cell health.

Q2: Can I use serum-containing medium during transfection?

A: Most polymer-based transfection reagents, including Hieff Trans™ Booster, are serum-compatible. However, avoid serum during complex formation; use serum-free medium (e.g., Opti-MEM) for that step.

Q3: What concentration should my mRNA stock be?

A: The mRNA concentration should be at least 100 ng/μL. For best results, use ≥ 0.5 μg/μL to minimize pipetting error.

Q4: How much mRNA should I use per well?

A: For a 6-well plate, we recommend 2–3 μg mRNA per well. Adjust accordingly for other formats (e.g., ~500–800 ng for 24-well).

Q5: How soon can I detect protein expression after transfection?

A: EGFP expression can typically be observed 6–12 hours post-transfection, with peak expression at 24–48 hours.

Q6: What should I do if transfection efficiency is low?

A: Ensure cells are healthy and at proper confluency.

  • Confirm mRNA quality: A260/A280 ~2.0, intact RNA (no degradation), and the presence of both a 5' cap and a 3' poly(A) tail. Increase the amount of mRNA used within a reasonable range.
  • Optimize the mRNA/reagent ratio: Adjust the mRNA/reagent ratio between 1:3 and 1:5 for optimal performance.
  • Control the incubation time of the complex: Incubate the complex for 5–10 minutes to avoid aggregation."
  • Optimize the detection time: Expression peaks may vary by cell type—commonly within 6–24 hours, but extended detection up to 48 hours may be required.

Related Products

Application

Name

Catalog No.

Size

Works with DNA, siRNA, miRNA, mRNA, and ASO, etc.

Proven success in primary cells.

Hieff TransTM Booster DNA&RNA Transfection Reagent

40801

100 μL/1.5 mL


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