Publication

High-throughput Microfluidic Platforms for S. cerevisiae Single Cell Studies

Hon Ming Andrew Yip
2022
Thèse EPFL
Résumé

Cells consume extra-cellular nutrients and resources to maintain cellular fitness. Extra-cellular conditions vary over time. Cellular programs encoded in genes adjust to adapt to the environments. Gene regulatory networks (GRNs) have evolved to be responsible for this task through regulation of a set of genes. The gene products work collectively, and assist cells to optimise their survival rate under nutrient limiting conditions. The PHO system is an example. It is a phosphate-responsive pathway found in S. cerevisiae. PHO genes are turned on when intra-cellular phosphate levels are limiting. The functions of individual genes in the PHO system are rather well-studied. However, the program that governs these genes at the system level is not yet fully understood. Systematic characterisation requires measurements of a large number of strains and environmental conditions. Conducting experiments while controlling consumable nutrients is especially challenging because the nutrient level decreases over time in a closed system. Chemostats allow stablilisation of nutrient levels, but have a lack of throughput. Conventional measurement instruments such as plate readers and cytometers do not satisfy experimental requirements including sub-cellular measurement, stable nutrient levels, and high throughput.Microfluidics is an experimental tool that is able to solve these bottlenecks. In this work, two microfluidic platforms were developed to satisfy the aforementioned requirements. With time-lapse fluorescence imaging, 1) single cell level measurement, 2) high strain and media condition throughput, 3) continuous media supply, and 4) temporally changing input control can be achieved by the proposed platforms. This work finely mapped the system response as a function of inorganic phosphate level. The sub-cellular localisation of the master transcription factor Pho4 and the PHO promoters' activities were studied at the single cell level under high resolution and well-controlled media conditions. Four program states were identified in the GRN and two promoter clusters were found. A new localisation state was also found in Pho4. These results resolved an outstanding question of how this system is programmed.

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Concepts associés (34)
Eutrophisation
thumb|upright=1.6|Les fertilisants utilisés pour les cultures (phosphore et azote) dopent la croissance des plantes et des algues dans le ru jouxtant le champ cultivé. En France et en Europe, la mise en place de zones-tampons est obligatoire le long des cours d'eau et des lacs. L'eutrophisation (du grec ancien : , « bien », et de , « nourriture ») est le processus par lequel des nutriments s'accumulent dans un milieu ou un habitat (terrestre ou aquatique).
Cycle des nutriments
vignette|Nutrient-cycle Le cycle des nutriments (ou recyclage écologique) est le processus par lequel les composés organiques et inorganiques sont réutilisés dans un nouveau but de production de la matière. A l'inverse, l'énergie est utilisée dans un but de consommation sans jamais revenir à son état de départ. On ne peut pas parler de cycle de l'énergie, contrairement au cycle des nutriments minéraux.
Cis-regulatory element
Cis-regulatory elements (CREs) or Cis''-regulatory modules (CRMs) are regions of non-coding DNA which regulate the transcription of neighboring genes. CREs are vital components of genetic regulatory networks, which in turn control morphogenesis, the development of anatomy, and other aspects of embryonic development, studied in evolutionary developmental biology. CREs are found in the vicinity of the genes that they regulate. CREs typically regulate gene transcription by binding to transcription factors.
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