Iron uptake of etioplasts is independent from photosynthesis but applies the reduction-based strategy

Máté Sági-Kazár; Éva Sárvári; Barnabás Cseh; Levente Illés; Zoltán May; Csaba Hegedűs; Attila Barócsi; Sándor Lenk; Katalin Solymosi; Ádám Solti

doi:10.3389/fpls.2023.1227811

Iron uptake of etioplasts is independent from photosynthesis but applies the reduction-based strategy

Front Plant Sci. 2023 Aug 11:14:1227811. doi: 10.3389/fpls.2023.1227811. eCollection 2023.

Authors

Affiliations

¹ Department of Plant Physiology and Molecular Plant Biology, Institute of Biology, ELTE Eötvös Loránd University, Budapest, Hungary.
² Doctoral School of Biology, Institute of Biology, ELTE Eötvös Loránd University, Budapest, Hungary.
³ Department of Plant Physiology, Umeå Plant Science Centre, Umeå University, Umeå, Sweden.
⁴ Department of Atomic Physics, Budapest University of Technology and Economics, Budapest, Hungary.
⁵ Institute of Materials and Environmental Chemistry, Research Centre for Natural Sciences, Eötvös Loránd Research Network, Budapest, Hungary.
⁶ Department of Plant Anatomy, Institute of Biology, ELTE Eötvös Loránd University, Budapest, Hungary.

Abstract

Introduction: Iron (Fe) is one of themost important cofactors in the photosynthetic apparatus, and its uptake by chloroplasts has also been associated with the operation of the photosynthetic electron transport chain during reduction-based plastidial Fe uptake. Therefore, plastidial Fe uptake was considered not to be operational in the absence of the photosynthetic activity. Nevertheless, Fe is also required for enzymatic functions unrelated to photosynthesis, highlighting the importance of Fe acquisition by non-photosynthetic plastids. Yet, it remains unclear how these plastids acquire Fe in the absence of photosynthetic function. Furthermore, plastids of etiolated tissues should already possess the ability to acquire Fe, since the biosynthesis of thylakoid membrane complexes requires a massive amount of readily available Fe. Thus, we aimed to investigate whether the reduction-based plastidial Fe uptake solely relies on the functioning photosynthetic apparatus.

Methods: In our combined structure, iron content and transcript amount analysis studies, we used Savoy cabbage plant as a model, which develops natural etiolation in the inner leaves of the heads due to the shading of the outer leaf layers.

Results: Foliar and plastidial Fe content of Savoy cabbage leaves decreased towards the inner leaf layers. The leaves of the innermost leaf layers proved to be etiolated, containing etioplasts that lacked the photosynthetic machinery and thus were photosynthetically inactive. However, we discovered that these etioplasts contained, and were able to take up, Fe. Although the relative transcript abundance of genes associated with plastidial Fe uptake and homeostasis decreased towards the inner leaf layers, both ferric chelate reductase FRO7 transcripts and activity were detected in the innermost leaf layer. Additionally, a significant NADP(H) pool and NAD(P)H dehydrogenase activity was detected in the etioplasts of the innermost leaf layer, indicating the presence of the reducing capacity that likely supports the reduction-based Fe uptake of etioplasts.

Discussion: Based on these findings, the reduction-based plastidial Fe acquisition should not be considered exclusively dependent on the photosynthetic functions.

Keywords: Blue Native polyacrylamide gel electrophoresis; chloroplast; ferric chelate reductase; thylakoid; x-ray fluorescence imaging.

Grants and funding

We acknowledge the financial support from the National Research, Development and Innovation Office, Hungary (NKFIH K-135607). MS-K was supported by the New National Excellence Program of the Ministry of Human Capacities, Hungary (ÚNKP-22-3-II-ELTE-755). Both SL, KS, and ÁS are grateful for their support by the Bolyai János Research Scholarship of the Hungarian Academy of Sciences. The XRF imaging facility at ELTE Eötvös Loránd University was granted by the European Structural and Investment Funds (VEKOP-2.3.3-15-2016-00008). The work of LI, AB, and SL on chlorophyll fluorescence lifetime measurements was supported by the Ministry of Culture and Innovation and the National Research, Development and Innovation Office within the Quantum Information National Laboratory of Hungary (Grant No. 2022-2.1.1-NL-2022-00004).