Biosimilars: SOP for Southern Blot Analysis – V 2.0
Standard Operating Procedure for Southern Blot Analysis in Biosimilar Cell Lines
| Department |
Biosimilars |
| SOP No. |
SOP/BS/018/2025 |
| Supersedes |
SOP/BS/018/2022 |
| Page No. |
Page 1 of 14 |
| Issue Date |
04/05/2025 |
| Effective Date |
06/05/2025 |
| Review Date |
04/05/2026 |
1. Purpose
To define the method for performing Southern blot analysis for confirming transgene integration, determining gene copy number, and detecting rearrangements in genetically modified biosimilar-producing cell lines.
2. Scope
This SOP applies to the Molecular Biology and Cell Line Development teams responsible for genetic characterization and verification of recombinant clones used in biosimilar production.
3. Responsibilities
- Molecular Biologist: Carries out the complete Southern blot procedure and interprets results.
- Lab Assistant: Prepares reagents, assists with electrophoresis and blotting steps.
- QA Representative: Verifies documentation and ensures traceability of results.
4. Accountability
The Head of Molecular Biology is accountable for ensuring the accurate execution and compliance of Southern blot assays as part of clone characterization in biosimilar programs.
5. Procedure
5.1 Genomic DNA Preparation
- Isolate high molecular weight DNA from 1 × 107 cells using phenol-chloroform extraction.
- Check DNA quality using agarose gel electrophoresis and spectrophotometry.
5.2 Restriction Enzyme Digestion
- Digest 10 µg genomic DNA with restriction enzymes that cut outside the transgene insertion site.
- Use at least 1 unit of enzyme per µg DNA and incubate overnight at 37°C.
5.3 Gel Electrophoresis and Denaturation
- Run digested DNA on 0.8% agarose gel at 40V overnight.
- Soak gel in 0.25M HCl for 10 minutes to depurinate.
- Denature in 1.5M NaCl, 0.5M NaOH for 30 minutes, followed by neutralization in 1.5M NaCl, 0.5M Tris-HCl pH 7.5.
5.4 Capillary Blotting
- Transfer DNA onto a nylon membrane overnight via capillary transfer in 20X SSC buffer.
- Cross-link DNA to membrane using UV crosslinker or baking at 80°C for 2 hours.
5.5 Probe Preparation and Hybridization
- Label the DNA probe (complementary to transgene) using radioactive or digoxigenin-based labeling.
- Prehybridize membrane in hybridization buffer for 1 hour at 42°C.
- Add labeled probe and hybridize overnight at 42–68°C depending on probe type.
5.6 Washing and Detection
- Wash membrane with decreasing stringency buffers (e.g., 2X SSC, 0.1X SSC).
- Detect signals using X-ray film (radioactive) or chemiluminescent substrate (DIG).
- Interpret number and intensity of bands to determine gene copy number and integration pattern.
- Document in Southern Blot Result Log (Annexure-1).
6. Abbreviations
- SSC: Saline-Sodium Citrate Buffer
- DIG: Digoxigenin
- UV: Ultraviolet
- X-ray: Radiographic Detection Method
7. Documents
- Southern Blot Result Log (Annexure-1)
- Probe Synthesis and Labeling Record (Annexure-2)
8. References
- WHO TRS 999 – Genetic Stability Testing of Cell Substrates
- ICH Q5B – Quality of Biotechnological Products: Analysis of Expression Constructs
- CDSCO Guidelines on Recombinant Cell Line Characterization
9. SOP Version
Version: 2.0
10. Approval Section
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Checked By |
Approved By |
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11. Annexures
Annexure-1: Southern Blot Result Log
| Date |
Clone ID |
Restriction Enzyme |
Band Count |
Band Size(s) |
Remarks |
Operator |
| 03/05/2025 |
CL-BS-018 |
EcoRI |
3 |
3.2kb, 2.8kb, 1.5kb |
Multiple integrations |
Rajesh Kumar |
Annexure-2: Probe Synthesis and Labeling Record
| Probe Name |
Target Gene |
Labeling Method |
Lot No. |
Prepared By |
Date |
| pEPO-3 |
rhEPO |
DIG |
DG2025 |
Sunita Reddy |
02/05/2025 |
Revision History:
| Revision Date |
Revision No. |
Revision Details |
Reason for Revision |
Approved By |
| 04/05/2025 |
2.0 |
Updated hybridization buffer and added DIG detection method |
Annual SOP update |
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