Seasonal Weather Changes Affect the Yield and Quality of Recombinant Proteins Produced in Transgenic Tobacco Plants in a Greenhouse Setting

Knödler, Matthias; Rühl, Clemens; Emonts, J.; Buyel, Johannes F.

doi:10.3389/fpls.2019.01245

Cited by 27 publications

(21 citation statements)

References 35 publications

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“…3 shows the growth rate “ r ( T )” values for a range of temperature. It confirms previously reported optimal growth range (18.5–28.5 °C) [7] which corresponds to 291.5–301.5 K.…”

Section: Experimental Design Materials and Methodssupporting

confidence: 92%

Techno-economic process modelling and Monte Carlo simulation data of uncertainty quantification in field-grown plant-based manufacturing

et al. 2021

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This data article is related to the research article, “ M.J. McNulty, K. Kelada, D. Paul, S. Nandi, and K.A. McDonald, Introducing uncertainty quantification to techno-economic models of manufacturing field-grown plant-made products, Food Bioprod. Process. 128 (2021) 153–165.” The raw and analyzed data presented are related to generation, analysis, and optimization of ultra-large-scale field-grown plant-based manufacturing of high-value recombinant protein under uncertainty. The data have been acquired using deterministic techno-economic process model simulation in SuperPro Designer integrated with stochastic Monte Carlo-based simulation in Microsoft Excel using the Crystal Ball plug-in. The purpose of the article is to make techno-economic and associated uncertainty data available to be leveraged and adapted for other research purposes.

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“…3 shows the growth rate “ r ( T )” values for a range of temperature. It confirms previously reported optimal growth range (18.5–28.5 °C) [7] which corresponds to 291.5–301.5 K.…”

Section: Experimental Design Materials and Methodssupporting

confidence: 92%

Techno-economic process modelling and Monte Carlo simulation data of uncertainty quantification in field-grown plant-based manufacturing

et al. 2021

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“…In the future, we will use mid-term and longterm cultures with more than 50% v/v D 2 O to increase the degree of 2 H labelling. Overall, our data show that plant cells offer a promising alternative to other eukaryotic systems for the high-level incorporation of deuterium in proteins, overcoming the toxicity issues affecting mammalian cells (Kushner et al, 1999). In addition to an estimation of the labelling degree, the mass spectrometry data can be used to assess the presence of post-translational modifications in plants versus E. coli.…”

Section: Analysis Of Plant-derived Gb1 By Esi-ms and Nmr Spectroscopymentioning

confidence: 89%

“…stained host cell proteins (HCPs) and GB1) in a sample were used to estimate GB1 purity. Samples were also analysed by dot blot (Opdensteinen et al, 2021) using ImageJ (Schneider et al, 2012) for quantitative comparison to His 6 -tagged GB1 standards at concentrations of 0.0, 1.5, 3.5, 7.5, 10.0, 20.0, 40 and 70.0 mg/ L. DsRed fluorescence in the expression controls was quantified as previously described using 12 standards in the 0-225 mg/L range (Kn ödler et al, 2019).…”

Section: Sample Analysismentioning

confidence: 99%

The transient expression of recombinant proteins in plant cell packs facilitates stable isotope labelling for NMR spectroscopy

Opdensteinen

Sperl

Mohamadi

et al. 2022

Plant Biotechnology Journal

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Summary Nuclear magnetic resonance (NMR) spectroscopy can be used to determine the structure, dynamics and interactions of proteins. However, protein NMR requires stable isotope labelling for signal detection. The cells used for the production of recombinant proteins must therefore be grown in medium containing isotopically labelled substrates. Stable isotope labelling is well established in Escherichia coli, but bacteria are only suitable for the production of simple proteins without post‐translational modifications. More complex proteins require eukaryotic production hosts, but their growth can be impaired by labelled media, thus reducing product yields and increasing costs. To address this limitation, we used media supplemented with isotope‐labelled substrates to cultivate the tobacco‐derived cell line BY‐2, which was then cast into plant cell packs (PCPs) for the transient expression of a labelled version of the model protein GB1. Mass spectrometry confirmed the feasibility of isotope labelling with 15N and 2H using this approach. The resulting NMR spectrum featured a signal dispersion comparable to recombinant GB1 produced in E. coli. PCPs therefore offer a rapid and cost‐efficient alternative for the production of isotope‐labelled proteins for NMR analysis, especially suitable for complex proteins that cannot be produced in microbial systems.

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“…[ 28 ] IgG1 and IgG3 antibodies were quantified by surface plasmon resonance (SPR) spectroscopy, using sensors coated with protein A (IgG1) or protein G (IgG3) and 2G12 as a standard, as previously described. [ 24 ] DsRed was quantified using eight standards in the 0 to 225 mg L ‐1 range as previously described [ 29 ] and the concentration of total soluble protein (TSP) was determined using eight dilutions of bovine serum albumin in the range 0 to 2000 mg L ‐1 as previously described. [ 30 ] Osmolality‐dependent DsRed expression was approximated using a log‐normal model (Equation 1):

\begin{equation}y = {y_0} + \frac{A}{{\sqrt {2\pi \cdot w\cdot x} }}{e^{\frac{{ - {{\left[ {\ln \frac{x}{{{x_c}}}} \right]}^2}}}{{2{w^2}}}}}\end{equation}

where y 0 is the minimal value ( y ‐offset) of the distribution (here, the minimal DsRed expression), x is the independent variable (here, the osmolality), x c is the center of the distribution, w is the standard deviation (width) of the distribution, and A is the area under the curve.…”

Section: Methodsmentioning

confidence: 99%

Reducing water uptake into BY‐2 cells by systematically optimizing the cultivation parameters increases product yields achieved by transient expression in plant cell packs

Opdensteinen

Buyel

2022

Biotechnology Journal

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Plant‐based production systems are inexpensive and easy to handle, allowing them to complement existing platforms for the production of protein‐based vaccines, therapeutics and diagnostic reagents. However, screening product candidates in whole plants requires a large facility footprint and is challenging due to natural variations in recombinant protein accumulation. In contrast, plant cell packs (PCPs) allow more than 1000 samples to be screened per day in microtiter plates. PCPs enable rapid development cycles based on transient expression in as little as 3 days, and yield milligram quantities of product for initial quality assessment and functional testing. However, this requires high‐level expression in BY‐2 cells and consistent cell quality across batches. We therefore used a statistical design of experiments (DoE) approach to systematically assess factors that contribute to consistent high yields of recombinant proteins in PCPs. Specifically, we tested the osmolality, pH, carbon source, light source, and additives during cell cultivation, as well as cell and PCP harvest times. The careful adjustment of these factors increased overall productivity by approximately fourfold. Remarkably all cultivation conditions leading to high productivities during transient expression in PCPs were associated with a reduced water uptake into the central vacuole. The universal presence of a vacuole in plant cells indicates that our results should be transferrable to other cells lines. Our findings therefore support the broad application of PCPs for screening and product analysis during the development of protein‐based pharmaceuticals and reagents in plants.

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Seasonal Weather Changes Affect the Yield and Quality of Recombinant Proteins Produced in Transgenic Tobacco Plants in a Greenhouse Setting

Cited by 27 publications

References 35 publications

Techno-economic process modelling and Monte Carlo simulation data of uncertainty quantification in field-grown plant-based manufacturing

Techno-economic process modelling and Monte Carlo simulation data of uncertainty quantification in field-grown plant-based manufacturing

The transient expression of recombinant proteins in plant cell packs facilitates stable isotope labelling for NMR spectroscopy

Reducing water uptake into BY‐2 cells by systematically optimizing the cultivation parameters increases product yields achieved by transient expression in plant cell packs

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