Coupling of on-column trypsin digestion-peptide mapping and principal component analysis for stability and biosimilarity assessment of recombinant human growth hormone

Sara M Shatat; Basma M Eltanany; Abeer A Mohamed; Medhat A Al-Ghobashy; Faten A Fathalla; Samah S Abbas

doi:10.1016/j.jchromb.2017.11.007

Coupling of on-column trypsin digestion-peptide mapping and principal component analysis for stability and biosimilarity assessment of recombinant human growth hormone

J Chromatogr B Analyt Technol Biomed Life Sci. 2018 Jan 1:1072:105-115. doi: 10.1016/j.jchromb.2017.11.007. Epub 2017 Nov 11.

Authors

Sara M Shatat¹, Basma M Eltanany², Abeer A Mohamed¹, Medhat A Al-Ghobashy³, Faten A Fathalla¹, Samah S Abbas²

Affiliations

¹ National Organization for Research and Control of Biologicals, Egypt.
² Analytical Chemistry Department, Faculty of Pharmacy, Cairo University, Egypt.
³ Analytical Chemistry Department, Faculty of Pharmacy, Cairo University, Egypt; Bioanalysis Research Group, School of Pharmacy, New Giza University, Egypt. Electronic address: medhat.alghobashy@cu.edu.eg.

PMID: 29145025
DOI: 10.1016/j.jchromb.2017.11.007

Abstract

Peptide mapping (PM) is a vital technique in biopharmaceutical industry. The fingerprint obtained helps to qualitatively confirm host stability as well as verify primary structure, purity and integrity of the target protein. Yet, in-solution digestion followed by tandem mass spectrometry is not suitable as a routine quality control test. It is time consuming and requires sophisticated, expensive instruments and highly skilled operators. In an attempt to enhance the fuctionality of PM and extract multi-dimentional data about various critical quality attributes and comparability of biosimilars, coupling of PM generated using immobilized trypsin followed by HPLC-UV to principal component analysis (PCA) is proposed. Recombinant human growth hormone (rhGH); was selected as a model biopharmaceutical since it is available in the market from different manufacturers and its PM is a well-established pharmacopoeial test. Samples of different rhGH biosimilars as well as degraded samples: deamidated and oxidized were subjected to trypsin digestion followed by RP-HPLC-UV analysis. PCA of the entire chromatograms of test and reference samples was then conducted. Comparison of the scores of samples and investigation of the loadings plots clearly indicated the applicability of PM-PCA for: i) identity testing, ii) biosimilarity assessment and iii) stability evaluation. Hotelling's T² and Q statistics were employed at 95% confidence level to measure the variation and to test the conformance of each sample to the PCA model, respectively. Coupling of PM to PCA provided a novel tool to identify peptide fragments responsible for variation between the test and reference samples as well as evaluation of the extent and relative significance of this variability. Transformation of conventional PM that is largely based on subjective visual comparison into an objective statiscally-guided analysis framework should provide a simple and economic tool to help both manufacturers and regulatory authorities in quality and biosimilarity assessment of biopharmaceuticals.

Keywords: Biosimilars; On-column trypsin digestion; Peptide mapping; Principal component analysis; Recombinant human growth hormone.

MeSH terms

Chromatography, Liquid
Ethylene Glycol / chemistry
Human Growth Hormone / analysis*
Human Growth Hormone / chemistry
Human Growth Hormone / metabolism
Limit of Detection
Linear Models
Peptide Fragments / analysis*
Peptide Fragments / chemistry
Peptide Fragments / metabolism
Peptide Mapping / methods*
Principal Component Analysis
Protein Stability
Recombinant Proteins / analysis*
Recombinant Proteins / chemistry
Recombinant Proteins / metabolism
Reproducibility of Results
Spectrometry, Mass, Electrospray Ionization
Trypsin / metabolism

Substances

Peptide Fragments
Recombinant Proteins
Human Growth Hormone
Trypsin
Ethylene Glycol