Quantitative evaluation of protocorm growth and fungal colonization in Bletilla striata (Orchidaceae) reveals less-productive symbiosis with a non-native symbiotic fungus

Tatsuki Yamamoto; Chihiro Miura; Masako Fuji; Shotaro Nagata; Yuria Otani; Takahiro Yagame; Masahide Yamato; Hironori Kaminaka

doi:10.1186/s12870-017-1002-x

Quantitative evaluation of protocorm growth and fungal colonization in Bletilla striata (Orchidaceae) reveals less-productive symbiosis with a non-native symbiotic fungus

BMC Plant Biol. 2017 Feb 21;17(1):50. doi: 10.1186/s12870-017-1002-x.

Authors

Tatsuki Yamamoto¹, Chihiro Miura², Masako Fuji², Shotaro Nagata¹, Yuria Otani¹, Takahiro Yagame³, Masahide Yamato⁴, Hironori Kaminaka⁵

Affiliations

¹ Graduate School of Agriculture, Tottori University, Tottori, Japan.
² Faculty of Agriculture, Tottori University, Tottori, Japan.
³ Tsukuba Botanical Garden, National Museum of Nature and Science, Tsukuba, Japan.
⁴ Faculty of Education, Chiba University, Chiba, Japan.
⁵ Faculty of Agriculture, Tottori University, Tottori, Japan. kaminaka@muses.tottori-u.ac.jp.

Abstract

Background: In nature, orchid plants depend completely on symbiotic fungi for their nutrition at the germination and the subsequent seedling (protocorm) stages. However, only limited quantitative methods for evaluating the orchid-fungus interactions at the protocorm stage are currently available, which greatly constrains our understanding of the symbiosis. Here, we aimed to improve and integrate quantitative evaluations of the growth and fungal colonization in the protocorms of a terrestrial orchid, Blettila striata, growing on a plate medium.

Results: We achieved both symbiotic and asymbiotic germinations for the terrestrial orchid B. striata. The protocorms produced by the two germination methods grew almost synchronously for the first three weeks. At week four, however, the length was significantly lower in the symbiotic protocorms. Interestingly, the dry weight of symbiotic protocorms did not significantly change during the growth period, which implies that there was only limited transfer of carbon compounds from the fungus to the protocorms in this relationship. Next, to evaluate the orchid-fungus interactions, we developed an ink-staining method to observe the hyphal coils in protocorms without preparing thin sections. Crushing the protocorm under the coverglass enables us to observe all hyphal coils in the protocorms with high resolution. For this observation, we established a criterion to categorize the stages of hyphal coils, depending on development and degradation. By counting the symbiotic cells within each stage, it was possible to quantitatively evaluate the orchid-fungus symbiosis.

Conclusions: We describe a method for quantitative evaluation of orchid-fungus symbiosis by integrating the measurements of plant growth and fungal colonization. The current study revealed that although fungal colonization was observed in the symbiotic protocorms, the weight of the protocorm did not significantly increase, which is probably due to the incompatibility of the fungus in this symbiosis. These results suggest that fungal colonization and nutrition transfer can be differentially regulated in the symbiosis. The evaluation methods developed in this study can be used to study various quantitative aspects of the orchid-fungus symbiosis.

Keywords: Bletilla striata; Germination; Mycorrhizal symbiosis; Orchid; Quantitative evaluation.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

DNA, Fungal / isolation & purification
Germination
Mycorrhizae / genetics
Mycorrhizae / physiology*
Orchidaceae / growth & development
Orchidaceae / microbiology*
Symbiosis*

Substances

DNA, Fungal