Maize cytolines as models to study the impact of different cytoplasms on gene expression under heat stress conditions

Ioana V Ardelean; Loredana Bălăcescu; Oana Sicora; Ovidiu Bălăcescu; Lia Mladin; Voichița Haș; Mihai Miclăuș

doi:10.1186/s12870-022-04023-8

Maize cytolines as models to study the impact of different cytoplasms on gene expression under heat stress conditions

BMC Plant Biol. 2023 Jan 2;23(1):4. doi: 10.1186/s12870-022-04023-8.

Authors

Ioana V Ardelean^{1

2}, Loredana Bălăcescu³, Oana Sicora¹, Ovidiu Bălăcescu³, Lia Mladin¹, Voichița Haș⁴, Mihai Miclăuș^{5

6}

Affiliations

¹ Biological Research Center, "Babeș-Bolyai" University, Jibou, Romania.
² NIRDBS, Institute of Biological Research, Cluj-Napoca, Romania.
³ The Oncology Institute "Prof Dr Ion Chiricuta", Cluj-Napoca, Romania.
⁴ Agricultural Research and Development Station, Turda, Romania.
⁵ NIRDBS, Institute of Biological Research, Cluj-Napoca, Romania. mihai.miclaus@icbcluj.ro.
⁶ STAR-UBB, "Babeș-Bolyai" University, Cluj-Napoca, Romania. mihai.miclaus@icbcluj.ro.

Abstract

Background: Crops are under constant pressure due to global warming, which unfolds at a much faster pace than their ability to adapt through evolution. Agronomic traits are linked to cytoplasmic-nuclear genome interactions. It thus becomes important to understand the influence exerted by the organelles on gene expression under heat stress conditions and profit from the available genetic diversity. Maize (Zea mays) cytolines allow us to investigate how the gene expression changes under heat stress conditions in three different cytoplasmic environments, but each having the same nucleus. Analyzing retrograde signaling in such an experimental set-up has never been done before. Here, we quantified the response of three cytolines to heat stress as differentially expressed genes (DEGs), and studied gene expression patterns in the context of existing polymorphism in their organellar genomes.

Results: Our study unveils a plethora of new genes and GO terms that are differentially expressed or enriched, respectively, in response to heat stress. We report 19,600 DEGs as responding to heat stress (out of 30,331 analyzed), which significantly enrich 164 GO biological processes, 30 GO molecular functions, and 83 GO cell components. Our approach allowed for the discovery of a significant number of DEGs and GO terms that are not common in the three cytolines and could therefore be linked to retrograde signaling. Filtering for DEGs with a fold regulation > 2 (absolute values) that are exclusive to just one of the cytolines, we find a total of 391 up- and down-DEGs. Similarly, there are 19 GO terms with a fold enrichment > 2 that are cytoline-specific. Using GBS data we report contrasting differences in the number of DEGs and GO terms in each cytoline, which correlate with the genetic distances between the mitochondrial genomes (but not chloroplast) and the original nuclei of the cytolines, respectively.

Conclusions: The experimental design used here adds a new facet to the paradigm used to explain how gene expression changes in response to heat stress, capturing the influence exerted by different organelles upon one nucleus rather than investigating the response of several nuclei in their innate cytoplasmic environments.

Keywords: Gene expression profiling; Heat-shock response; Organelles; Retrograde signaling; Zea mays.

MeSH terms

Cytoplasm / genetics
Gene Expression
Gene Expression Profiling
Gene Expression Regulation, Plant
Heat-Shock Response* / genetics
Phenotype
Zea mays* / metabolism