One goal of the 2018 iGEM Interlab study is to overcome the weakness inherent in the commonly-used measurement of promoter strength, that of reporting the fluorescence value relative to the optical density at 600 nm (OD₆₀₀ nm) of the culture media. There is clearly the potential for a discrepancy to occur between OD₆₀₀ nm and actual cell concentration which can result in an erroneous conclusion being drawn about the effectiveness of the promoter. This year the 2018 iGEM study sought to reduce lab-to-lab variability by measuring GFP fluorescence relative to absolute cell counts or colony forming units (cfu). Normalisation of fluorescence against cfu ensures measurement of fluorescence relative only to viable cells.

Our RFP internal standard (IS) was developed to address the issue that copy number of the same plasmid is not consistent across cells. The inclusion of an IS RFP signal [Figure 1 http://parts.igem.org/Part:BBa_K2797013] is therefore designed to allow measurement of variation in gene expression between cultures and transformant lines. The underpinning assumption is that because the IS devices are identical across each of the plasmids, the GFP fluorescence values of the test devices of interest can be reported relative to their internal RFP signal.

The new plasmids were tested. Analysis of the internal standards involved comparing the original InterLab test device plasmid performance against the new internal standard plasmid performance. MTP wells A-D represented the E. coli containin the RFP internal standard vector and wells E-H represented E. coli containing the original test devices. Column 9 wells A-H contained an LB+cam blank. The microtiter plate was incubated for 24 hours in the plate reader with Abs600, fluorescence (GFP): Excitation 485, Emission 420 and fluorescence; (RFP): Excitation 588, emission 635 measured every 15 minutes following a short shake at 420 rpm at a low shake diameter.

Although there was no calibration standard available for our RFP, there was a clear indication that there was variation in RFP gene expression between each device [Figure 2]. It is important to remember that the only genetic difference between these devices is in the promoter used to drive GFP expression - not RFP expression. Moreover, the inclusion of the RFP impacted on the response of the GFP signals across the test devices. GFP fluorescence values of the modified Interlab plasmids were seen to be lower than standard Interlab devices. Devices 1 & 4 – the devices with the strongest promoters – exhibited lower GFP fluorescence than unmodified Interlab plasmids and did not show any RFP fluorescence (sequencing confirmed the presence of the RFP part). Taken together these observations suggest that there is competition for cellular resources (i.e. Transcriptional/translational machinery) [6].This has been observed previously in E. coli, where genes are activated and deplete the pool of free RNAP and ribosomes, reducing their availability to other cassettes [7,8]. In this case, it may be that gene expression of GFP in devices 1 & 4 is so powerful that there is no available cellular machinery to enable protein synthesis whilst the variation in RFP signals across all plasmids is likely to result from similar, but less pronounced competition.

A further interesting observation is the difference seen in GFP signal longevity. The fluorescence/OD600nm of the original test devices exhibited a significant decrease after six hours while in the IS containing devices, although the signal was lower, it remained more consistent over 24 hours. Genes have been known to act as transcriptional modulators for one another in the same operon [10]. However, genes on the same plasmid but at different locations can act as transcriptional modulators for one another [6]. It may be that a coupling of these genes due to competition for transcriptional machinery has led to the modulation of GFP gene expression, causing it to be less productive but more consistent. There is room for improvement in this study. RFP is a slow maturing protein. Fluorescent proteins like mCherry, which possess brighter fluorescence and fold faster than [11] are a better option for use as an IS. Furthermore, a calibration with a red fluorescent compound (e.g. rhodamine red) would be beneficial. This would allow ‘molecules of equivalent rhodamine red’ values so estimate RFP or other internal standard concentrations in cells.