HEK293 Host Cell DNA Residue Detection Kit (3G) Validation Report

HEK293 Host Cell DNA Residue Detection Kit (3G)

Qualification Summary (Cat No.: 41331ES60)

  1. Background

The data summarized in this report are performed by Yeasen Biotechnology for 'HEK293 Host Cell DNA Residue Detection Kit (3G)' product. The summary data is only for the user's reference, and the user needs to verify the host cell residue DNA method by using their own samples to confirm the method can meet the user's requirements. All laboratories who using this kit are recommended to verify the following parameters: Linearity, Range, Accuracy, Precision, Quantitation Limit, Specificity, and Robustness.

Yeasen Biotechnology can provide the detailed qualification report for this kit. If the user uses this report, then only the suitability (which included Precision, Accuracy and Specificity) should be verified.

  1. Experimental materials and methods

2.1 HEK293 Host Cell DNA Residue Detection Kit (3G), Vendor: Yeasen, Cat No.: 41331ES60.

2.2 MolPure® Magnetic Residual DNA Sample Preparation Kit, Vendor: Yeasen, Cat No.: 18461ES60.

2.3 Original data: the electronic version were recorded in the 'Experimental Report' the subfile of the parent file 'HEK293 Host Cell DNA Residue Detection Kit (3G)'.

2.4 Methods: The materials and operation methods used for the experiment were basically produced or set by Yeasen Biotechnology, which were assessed and verified for a long time, the kit development and manufacture are followed the ISO 13485 system.

  1. Qualification contents and results

3.1 Detection range

The linear range of the kit was 30 fg/μL~300 pg/μL with R2≥0.998, and the amplification efficiency was 90%~110% range with CV<15% for each concentration assay.

 

Figure 1 HEK293 DNA (3G) qPCR Standard Curve

3.2 Accuracy

3.2.1 Recovery

3.2.1.1 Blank Sample Spiking Recovery Experiment

Samples of HEK293 DNA standards at high and low concentrations: 300 pg/μL, 3 pg/μL, and 30 fg/μL were prepared, respectively, and assayed after extraction using the Magnetic Bead Method for Residual DNA Sample Pre-treatment Kit (2 extraction replicates were performed for each sample, and 3 assay replicates were done for each extraction), and the sample recoveries and CVs were analyzed.

For different concentrations of DNA samples, the recoveries ranged from 70% to 130%, and the CVs were all <20%.

Sample type

Theoretical Concentration

Extract 1 mean

Extract 2 mean

Average concentration

CV

Recovery

Blank Sample

/

/

/

/

/

/

Recovery sample 1

300 pg/μL

306.81 pg/μL

279.57 pg/μL

293.82 pg/μL

6.56%

97.94%

Recovery sample 2

3 pg/μL

3.11 pg/μL

2.99 pg/μL

3.09 pg/μL

2.75%

103.00%

Recovery sample 3

30 fg/μL

31.02 fg/μL

30.63 fg/μL

30.83 fg/μL

0.89%

102.77%

Table1 Blank Sample Spiking Recovery

3.2.1.2 Simulated Sample Spiking Recovery Experiment

Samples of the same concentration (3 pg/μL of HEK293 DNA) were extracted (2 extraction replicates were performed for each sample and 3 assay replicates were done for each extraction) with 5 different background solutions (high protein, high nucleic acid, high and low pH, high salt) and sample recoveries and CVs were analyzed.

DNA sample recoveries for different background solutions ranged from 70% to 130%, with all CVs <20%.

Sample type

Theoretical Concentration

Extract 1 mean

Extract 2 mean

Average concentration

CV

Recovery

Basic Sample

/

/

/

/

/

/

High Protein

3 pg/μL

2.65

2.80

2.73

3.80%

90.87%

High Nuclear Acid

2.82

2.97

2.90

3.71%

96.58%

High-salt

2.88

2.70

2.79

4.47%

92.89%

High pH

2.81

2.93

2.87

2.98%

95.71%

Low pH

2.76

2.79

2.77

0.99%

92.48%

Table2 Basic Sample Spiking Recovery

3.3 Precision

3.3.1 Repeatability

Repeat the assay 10 times for HEK293 DNA standards at a concentration of 30 fg/μL with a CV <15%.

Repetitions

1

2

3

4

5

6

7

8

9

10

Mean

CV%

Detection Value (fg/μL)

29.51

30.02

30.13

30.16

27.99

31.01

31.05

30.95

31.02

29.86

30.17

3.15%

Table3 Repeatability Results

3.3.2 Intermediate precision

Three experimenters independently tested HEK293 DNA standard samples at high and low concentrations: 300 pg/μL, 3 pg/μL, and 30 fg/μL, and three replicates were done for each concentration, and the CVs of all nine data obtained were <15%.

Exp

 

 

Actual Concentration

Theoretical Concentration

HEK293 DNA (3G)

300 pg/uL

3 pg/uL

30 fg/uL

Exp 1

Determination 1

319.58

3.026

32.02

Determination 2

309.76

3.051

37.01

Determination 3

309.24

3.067

36.03

Exp 2

Determination 4

308.34

2.909

29.91

Determination 5

308.54

2.9

29.67

Determination 6

305.83

2.921

28.85

Exp 3

Determination 7

299.11

3.035

29.36

Determination 8

300.07

2.833

31.14

Determination 9

302.03

3.033

33.07

/

Mean

306.95

2.975

31.90

/

CV%

2.03%

2.83%

9.26%

Table4 Intermediate precision Results

3.4 Specificity

The interference of cellular genomic DNA commonly used in the production of biologics was assessed for interference with HEK293 DNA detection reagents, and the interference group overlapped with the control group and no interference was seen (the figure below shows, in order, the interference data of CHO, E.coli, and Pichia Pastoris genomic DNAs with HEK293 DNA detection reagents).

    

Figure 2 Interference experiment results

3.5 Quantitation Limit

HEK293 DNA was detected at 30 fg/μL, 20 fg/μL, 10 fg/μL and 5 fg/μL, with 10 replicates for each concentration. The results showed that the CV was <20% at concentrations of 10 fg/μL and above. That is, the limit of quantification of the HEK293 host cell DNA residue detection kit (3G) was 10 fg/μL.

 

Repetitions

Test Item

HEK293 DNA (3G) (fg/μL)

Quantity

Recalculation Ratio%

1

11.04

110.40%

2

9.97

99.70%

3

11.12

111.20%

4

11.07

110.70%

5

11.21

112.10%

6

9.93

99.30%

7

10.25

102.50%

8

10.16

101.60%

9

10.08

100.80%

10

10.11

101.10%

Mean

10.49

/

CV%

5.14%

/

  

 

                                Figure 3 10fg/μL HEK293 DNA (3G) qPCR Test Result

3.6 Robustness

This kit has been tested and is suitable for, but not limited to, the following instruments:

Vendor

Instrument Models

Amplification Efficiencies

R2

Limit of quantification (fg/μL)

CV%

Thermo

ABI 7500

102.84%

1

10

7%

Thermo

ABI QuantStudio5

104.70%

0.999

10

9%

Shanghai Hongshi

SLAN

101.46%

0.999

10

8%

Table5 Instrument suitability test results

3.7 Stability

3.7.1 Freeze-thaw stability

HEK293 Host Cell DNA Residue Detection Kit (3G) was tested by repeated freezing and thawing 10 times, and the performance of the kit was not affected.

 

 

Testing Indicators

Freeze-thaw Times

Parameter

T0 time

Freeze-thaw 10 times

Standard Curve Parameter

Amplification Efficiencies

99.34%

100.78%

R2

1

1

Limit of quantification (30 fg/μL)

CV

11%

7%

Table6 Freeze-thaw stability result analysis

3.7.2 Accelerated Stability

HEK293 Host Cell DNA Residue Detection Kit (3G) were stored at 2~8°C for 30 days and 37°C for 14 days, respectively. None of the performance of the kit was affected.

 

 

Testing Indicators

Acceleration Temperature & Time

Parameter

T0 time

37℃ 7 Days

37℃ 14 Days

Standard Curve Parameter

Amplification Efficiencies

103.83%

101.58%

100.47%

R2

0.999

1

1

Limit of quantification (30 fg/μL)

CV%

8%

5%

5%

Table7 Accelerated stability result analysis

3.8 Limit of Blank

No template control (NTC) was a template dilution with 96 repetitions of CT values >32 (plus ROX calibration threshold line set to 0.06).

 

 

Figure 4 NTC experiment results

  1. 4.Reference

4.1 Chinese Pharmacopoeia Commission (ChPC). Pharmacopoeia of People's Republic of China (Vol Ⅲ) [S]. Beijing:China Medical Science and Technology Press,p.542-543, 2020.

4.2 NMPA, 2007: General Principles for Technical Review of Analytical Method Validation for Quality Control of Biological Products.

4.3 ICH(2022)《Analytical method validation Q2》, draft version.

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