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Analysis of Oligonucleotide Impurities on the BioAccord System with ACQUITY Premier

Applications | 2021 | WatersInstrumentation
LC/TOF, LC/HRMS, LC/MS
Industries
Pharma & Biopharma
Manufacturer
Waters

Summary

Significance of the Topic



Oligonucleotide-based therapeutics have emerged as a transformative class of drugs due to their high specificity and versatility. Ensuring the purity and accurate mass confirmation of heavily modified sequences is essential for safety, efficacy, and regulatory compliance. Impurity profiling at trace levels (<0.2%) is critical in both development and manufacturing environments.

Objectives and Study Overview



This study evaluates an automated, compliance-ready LC–MS workflow on the BioAccord System equipped with ACQUITY Premier. The primary goals are to confirm the intact mass of a 21-mer oligonucleotide featuring extensive 2′-OMe and 5-Me modifications, and to detect and quantify low-level impurities down to 0.2% relative abundance.

Methodology



Separation was carried out using ion-pairing reversed-phase UPLC with HFIP/TEA buffers and methanol gradients at 60 °C and 300 µL/min. A 21-mer sample (1 µM) was injected (10 µL, 10 pmol) onto ACQUITY Premier OST columns. MS detection used ESI in negative mode, full-scan (400–5000 m/z, 2 Hz). Data were processed via BayesSpray charge deconvolution in waters_connect for accurate average mass determination.

Instrumentation Used


  • BioAccord System with ACQUITY Premier UPLC BSM
  • ACQUITY Premier OST Columns (2.1×100 mm and 2.1×50 mm, 1.7 µm, 130 Å)
  • ACQUITY Tunable UV Detector
  • ESI-Tof ACQUITY RDa Mass Detector
  • waters_connect software (acquisition and processing)

Main Results and Discussion



Comparison between Premier and conventional columns demonstrated significant improvements:
  • Detection of 14 impurities on Premier versus 7 on conventional, illustrating reduced adsorption by MaxPeak HPS coatings.
  • Impurity quantification down to 0.18% abundance with mass accuracy better than 15 ppm across a ~500-fold dynamic range.
  • Reproducible UV peak areas (RSD <15%) at 0.5 nM (5 fmol) loading.
  • Linear UV calibration over three orders of magnitude (0.5–1000 nM, R²>0.99) and negligible carryover.

Benefits and Practical Applications


  • High sensitivity and minimal non-specific binding enable reliable profiling of therapeutic oligonucleotides.
  • Compliance-ready workflows ensure traceable, auditable data for regulated environments.
  • Accurate intact mass confirmation accelerates identity verification and quality control in R&D and manufacturing.

Future Trends and Potential Applications



Advances in inert-surface UPLC integrated with high-resolution MS and ion mobility promise enhanced separation of isobaric impurities. Expansion to high-throughput platforms and real-time compliance frameworks will further streamline analytical pipelines for biopolymer characterization.

Conclusion



The BioAccord System with ACQUITY Premier delivers a robust, sensitive, and reproducible workflow for oligonucleotide impurity analysis. MaxPeak HPS technology effectively mitigates metal surface interactions, allowing detection of impurities down to 0.2% and providing mass accuracy better than 15 ppm.

References


  1. Sharma VK, Watts JK. Oligonucleotide Therapeutics: Chemistry, Delivery and Clinical Progress. Future Med Chem. 2015;7(16):2221–2242.
  2. Roberts TK, Langer R, Wood MJA. Advances in Oligonucleotide Drug Delivery. Nat Rev Drug Discov. 2020;19:673–694.
  3. Doneanu CE, Fox J, Harry E, Knowles C, Yu YQ, Fredette J, Chen W. Automated Compliance-Ready LC–MS Workflow for Intact Mass Confirmation and Purity Analysis of Oligonucleotides. Waters Application Note. 2020;720006820EN.
  4. Lauber MA, Walter TH, Gilar M, et al. Low Adsorption HPLC Columns Based on MaxPeak High Performance Surfaces. Waters White Paper. 2020;720006930EN.
  5. Delano M, Walter TH, Lauber MA, et al. Mitigation of Analyte Loss on Metal Surfaces in UHPLC. Anal Chem. 2021;93:5773–5781.

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