| Literature DB >> 34097703 |
Jacob Beal1, Geoff S Baldwin2, Natalie G Farny3, Markus Gershater4, Traci Haddock-Angelli5, Russell Buckley-Taylor2, Ari Dwijayanti2, Daisuke Kiga6, Meagan Lizarazo5, John Marken7, Kim de Mora5, Randy Rettberg5, Vishal Sanchania4, Vinoo Selvarajah5, Abigail Sison5, Marko Storch8, Christopher T Workman9.
Abstract
Reproducibility is a key challenge of synthetic biology, but the foundation of reproducibility is only as solid as the reference materials it is built upon. Here we focus on the reproducibility of fluorescence measurements from bacteria transformed with engineered genetic constructs. This comparative analysis comprises three large interlaboratory studies using flow cytometry and plate readers, identical genetic constructs, and compatible unit calibration protocols. Across all three studies, we find similarly high precision in the calibrants used for plate readers. We also find that fluorescence measurements agree closely across the flow cytometry results and two years of plate reader results, with an average standard deviation of 1.52-fold, while the third year of plate reader results are consistently shifted by more than an order of magnitude, with an average shift of 28.9-fold. Analyzing possible sources of error indicates this shift is due to incorrect preparation of the fluorescein calibrant. These findings suggest that measuring fluorescence from engineered constructs is highly reproducible, but also that there is a critical need for access to quality controlled fluorescent calibrants for plate readers.Entities:
Year: 2021 PMID: 34097703 DOI: 10.1371/journal.pone.0252263
Source DB: PubMed Journal: PLoS One ISSN: 1932-6203 Impact factor: 3.240