In vivo expression vector derived from anhydrobiotic tardigrade genome enables live imaging in Eutardigrada

Author:

Tanaka Sae12ORCID,Aoki Kazuhiro234ORCID,Arakawa Kazuharu1256ORCID

Affiliation:

1. Institute for Advanced Biosciences, Keio University, Tsuruoka, 997-0017, Japan

2. Exploratory Research Center on Life and Living Systems, National Institutes of Natural Sciences, Okazaki, 444-8787, Japan

3. National Institute for Basic Biology, National Institutes of Natural Sciences, Okazaki, 444-8787, Japan

4. Faculty of Life Science, Graduate University for Advanced Studies, Okazaki, 444-8787, Japan

5. Graduate School of Media and Governance, Keio University, Fujisawa, 252-0882, Japan

6. Faculty of Environment and Information Studies, Keio University, Fujisawa, 252-0882, Japan

Abstract

Water is essential for life, but anhydrobiotic tardigrades can survive almost complete dehydration. Anhydrobiosis has been a biological enigma for more than a century with respect to how organisms sustain life without water, but the few choices of genetic toolkits available in tardigrade research have been a challenging circumstance. Here, we report the development of an in vivo expression system for tardigrades. This transient transgenic technique is based on a plasmid vector (TardiVec) with promoters that originated from an anhydrobiotic tardigrade Ramazzottius varieornatus . It enables the introduction of GFP-fused proteins and genetically encoded indicators such as the Ca 2+ indicator GCaMP into tardigrade cells; consequently, the dynamics of proteins and cells in tardigrades may be observed by fluorescence live imaging. This system is applicable for several tardigrades in the class Eutardigrada: the promoters of anhydrobiosis-related genes showed tissue-specific expression in this work. Surprisingly, promoters functioned similarly between multiple species, even for species with different modes of expression of anhydrobiosis-related genes, such as Hypsibius exemplaris, in which these genes are highly induced upon facing desiccation, and Thulinius ruffoi , which lacks anhydrobiotic capability. These results suggest that the highly dynamic expression changes in desiccation-induced species are regulated in trans . Tissue-specific expression of tardigrade-unique unstructured proteins also suggests differing anhydrobiosis machinery depending on the cell types. We believe that tardigrade transgenic technology opens up various experimental possibilities in tardigrade research, especially to explore anhydrobiosis mechanisms.

Funder

MEXT | Japan Society for the Promotion of Science

MEXT | NINS | Exploratory Research Center on Life and Living Systems, National Institutes of Natural Sciences

Yamagata Prefectural Government and Tsuruoka City

Publisher

Proceedings of the National Academy of Sciences

Subject

Multidisciplinary

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