Protoplast isolation from Dictyopteris pacifica and Scytosiphon lomentaria, using a simple commercial enzyme preparation

Jose Avila-Peltroche; Boo Yeon Won; Tae Oh Cho

doi:10.1186/s43141-021-00226-y

Protoplast isolation from Dictyopteris pacifica and Scytosiphon lomentaria, using a simple commercial enzyme preparation

J Genet Eng Biotechnol. 2021 Sep 3;19(1):135. doi: 10.1186/s43141-021-00226-y.

Authors

Jose Avila-Peltroche^{1

2}, Boo Yeon Won¹, Tae Oh Cho^{3

4}

Affiliations

¹ Department of Life Science, Chosun University, Gwangju, 61452, Korea.
² Department of Integrative Biological Sciences & BK21 FOUR Educational Research Group for Age-associated Disorder Control Technology, Chosun University, Gwangju, 61452, Korea.
³ Department of Life Science, Chosun University, Gwangju, 61452, Korea. tocho@chosun.ac.kr.
⁴ Department of Integrative Biological Sciences & BK21 FOUR Educational Research Group for Age-associated Disorder Control Technology, Chosun University, Gwangju, 61452, Korea. tocho@chosun.ac.kr.

Abstract

Background: Protoplasts (i.e., naked plant cells) can be used for in vitro manipulations and genetic improvement in cultivars with economic value. During the last decade, protoplast research in economic brown algae has been scarce, and it is usually hampered by the use of non-commercial enzymes or crude extracts for isolating protoplasts. Dictyopteris pacifica is part of a brown algal genus well known by its wide chemical diversity and biological properties. Scytosiphon lomentaria is an edible brown seaweed with antioxidant, antitumor, and antiviral properties. So far, there are no protoplast isolation protocols using commercial enzymes for these two economic brown algae. In this study, we obtained protoplasts from cultured samples of D. pacifica and S. lomentaria using commercially available enzymes. Additionally, we investigated the effects of Driselase inclusion and Ca-chelation pre-treatment on protoplast yields in order to optimize the conditions for protoplast preparations.

Results: Protoplasts were isolated from Dictyopteris pacifica and Scytosiphon lomentaria using the commercially available Cellulase Onozuka RS (1%) and Alginate lyase (4 U mL^-1), and short incubation time (4 h). Driselase did not show significant effects on protoplast production in both species. Ca-chelation pre-treatment only increased the number of protoplasts in D. pacifica. Under optimal conditions, the protoplast yields from D. pacifica and S. lomentaria were 4.83 ± 2.08 and 74.64 ± 32.49 × 10⁶ protoplasts g^-1 fresh weight, respectively. The values obtained for S. lomentaria were 2-3 orders of magnitude higher than previously reported.

Conclusions: Our results show that high protoplast yields can be obtained from D. pacifica and S. lomentaria using a simple mixture of commercial enzymes (Cellulase RS and Alginate lyase) and short incubation time (4 h). This work also represents the first report of protoplast isolation in D. pacifica. The method proposed here can help to expand protoplast technology in more brown algal species.

Keywords: Brown algae; Commercial enzymes; Cultured samples; Dictyopteris pacifica; Protoplast isolation; Scytosiphon lomentaria.

Abstract

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