Time Is a Critical Factor When Evaluating Oligonucleotide Therapeutics in hERG Assays

Yusheng Qu; Robert Kirby; Richard Davies; Ayesha Jinat; Stefano Stabilini; Bin Wu; Longchuan Yu; BaoXi Gao; Hugo M Vargas

doi:10.1089/nat.2022.0043

Time Is a Critical Factor When Evaluating Oligonucleotide Therapeutics in hERG Assays

Nucleic Acid Ther. 2023 Apr;33(2):132-140. doi: 10.1089/nat.2022.0043. Epub 2022 Dec 26.

Authors

Yusheng Qu¹, Robert Kirby², Richard Davies², Ayesha Jinat², Stefano Stabilini², Bin Wu³, Longchuan Yu⁴, BaoXi Gao¹, Hugo M Vargas¹

Affiliations

¹ Amgen Research, Translational Safety and Bioanalytical Sciences, Amgen, Inc., Thousand Oaks, California, USA.
² Metrion Biosciences Ltd, Granta Center, Cambridge, United Kingdom.
³ Hybrid Modality Engineering, Amgen, Inc., Thousand Oaks, California, USA.
⁴ Cardiometabolic Disorders, Amgen, Inc., Thousand Oaks, California, USA.

Abstract

In accord with International Conference on Harmonization S7B guidelines, an in vitro human ether-a-go-go-related gene (hERG) assay is one component of an integrated risk assessment for delayed ventricular repolarization. Function of hERG could be affected by direct (acute) mechanisms, or by indirect (chronic) mechanisms. Some approved oligonucleotide therapeutics had submitted hERG data to regulatory agents, which were all collected with the same protocol used for small-molecule testing (incubation time <20 min; acute), however, oligonucleotides have unique mechanisms and time courses of action (indirect). To reframe the hERG testing strategy for silencing RNA (siRNA), an investigation was performed to assess the time course for siRNA-mediated inhibition of hERG function and gene expression. Commercially available siRNAs of hERG were evaluated in a stable hERG-expressed cell line by whole-cell voltage clamp using automated electrophysiology and polymerase chain reaction. In the acute hERG study, no effects were observed after treatment with 100 nM siRNA for 20 min. The chronic effects of 100 nM siRNAs on hERG function were evaluated and recorded over 8-48 h following transfection. At 8 h there was no significant effect, whereas 77% reduction was observed at 48 h. Measurement of hERG mRNA levels demonstrated a 79% and 93% decrease of hERG mRNA at 8 and 48 h, respectively, consistent with inhibition of hERG transcription. The results indicate that an anti-hERG siRNA requires a long exposure time (48 h) in the hERG assay to produce a maximal reduction in hERG current; short exposures (20 min-8 h) had no effect. These findings imply that off-target profiling of novel oligonucleotides could benefit from using hERG protocol with long incubation times to de-risk potential off-target (indirect) effects on the hERG channel. This hERG assay modification may be important to consider if the findings are used to support an integrated nonclinical-clinical risk assessment for QTc (the duration of the QT interval adjusted for heart rate) prolongation.

Keywords: PCR; automated electrophysiology; hERG; oligonucleotide; siRNA.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Cell Line
Ether-A-Go-Go Potassium Channels* / genetics
Ether-A-Go-Go Potassium Channels* / metabolism
Humans
RNA, Small Interfering / genetics

Substances

Ether-A-Go-Go Potassium Channels
RNA, Small Interfering