High-Throughput Cryopreservation of Plant Cell Cultures for Functional Genomics

Ogawa, Yoichi; Sakurai, Nozomu; Oikawa, Akira; Kai, Kosuke; Morishita, Yoshihiko; Mori, Ken-ichiro; Moriya, Kensuke; Fujii, Fumiko; Aoki, Koh; Suzuki, Hideyuki; Ohta, Daisaku; Saito, Kazuki; Shibata, Daisuke

doi:10.1093/pcp/pcs038

Cited by 40 publications

(22 citation statements)

References 24 publications

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“…Continuous culturing of transgenic plant cells frequently resulted in the loss of transgene functions or reduced cell viability. Recently, cryopreservation procedures for various plant cells have been developed [ 27 , 28 ]. We thus attempted to establish a procedure for sodium alginate-based cryopreservation of F .…”

Section: Resultsmentioning

confidence: 99%

“…Cryopreservation of F . koreana wildtype and transgenic cells was tested under various conditions using sodium alginate based on previous reports with various modifications [ 27 , 28 ]. U18i-CPi-Fk was centrifuged at 100 x g for 5 min, and was then resuspended in Gamborg’s B-5 medium containing 2% (w/v) sodium alginate, with cell density of 5 x 10 6 / ml.…”

Section: Methodsmentioning

confidence: 99%

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Generation of Triple-Transgenic Forsythia Cell Cultures as a Platform for the Efficient, Stable, and Sustainable Production of Lignans

et al. 2015

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Sesamin is a furofuran lignan biosynthesized from the precursor lignan pinoresinol specifically in sesame seeds. This lignan is shown to exhibit anti-hypertensive activity, protect the liver from damages by ethanol and lipid oxidation, and reduce lung tumor growth. Despite rapidly elevating demand, plant sources of lignans are frequently limited because of the high cost of locating and collecting plants. Indeed, the acquisition of sesamin exclusively depends on the conventional extraction of particular Sesamum seeds. In this study, we have created the efficient, stable and sustainable sesamin production system using triple-transgenic Forsythia koreana cell suspension cultures, U18i-CPi-Fk. These transgenic cell cultures were generated by stably introducing an RNAi sequence against the pinoresinol-glucosylating enzyme, UGT71A18, into existing CPi-Fk cells, which had been created by introducing Sesamum indicum sesamin synthase (CYP81Q1) and an RNA interference (RNAi) sequence against pinoresinol/lariciresinol reductase (PLR) into F. koreanna cells. Compared to its transgenic prototype, U18i-CPi-Fk displayed 5-fold higher production of pinoresinol aglycone and 1.4-fold higher production of sesamin, respectively, while the wildtype cannot produce sesamin due to a lack of any intrinsic sesamin synthase. Moreover, red LED irradiation of U18i-CPi-Fk specifically resulted in 3.0-fold greater production in both pinoresinol aglycone and sesamin than production of these lignans under the dark condition, whereas pinoresinol production was decreased in the wildtype under red LED. Moreover, we developed a procedure for sodium alginate-based long-term storage of U18i-CPi-Fk in liquid nitrogen. Production of sesamin in U18i-CPi-Fk re-thawed after six-month cryopreservation was equivalent to that of non-cryopreserved U18i-CPi-Fk. These data warrant on-demand production of sesamin anytime and anywhere. Collectively, the present study provides evidence that U18i-CP-Fk is an unprecedented platform for efficient, stable, and sustainable production of sesamin, and shows that a transgenic and specific light-regulated Forsythia cell-based metabolic engineering is a promising strategy for the acquisition of rare and beneficial lignans.

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Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Generation of Triple-Transgenic Forsythia Cell Cultures as a Platform for the Efficient, Stable, and Sustainable Production of Lignans

et al. 2015

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“…Arabidopsis cell lines have been cryogenically frozen at −30 °C or −80 °C and then thawed out, and the cell activity remained similar to unfrozen cells [103]. A similar experiment was also performed in transgenic rice expressing recombinant hCTLA4Ig and cells recovered from cryopreservation banking had cell viability of 88% [102].…”

Section: Improvement Of Rice Expression Systemmentioning

confidence: 99%

Improving Pharmaceutical Protein Production in Oryza sativa

Kuo

Tan

et al. 2013

IJMS

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Application of plant expression systems in the production of recombinant proteins has several advantages, such as low maintenance cost, absence of human pathogens, and possession of complex post-translational glycosylation capabilities. Plants have been successfully used to produce recombinant cytokines, vaccines, antibodies, and other proteins, and rice (Oryza sativa) is a potential plant used as recombinant protein expression system. After successful transformation, transgenic rice cells can be either regenerated into whole plants or grown as cell cultures that can be upscaled into bioreactors. This review summarizes recent advances in the production of different recombinant protein produced in rice and describes their production methods as well as methods to improve protein yield and quality. Glycosylation and its impact in plant development and protein production are discussed, and several methods of improving yield and quality that have not been incorporated in rice expression systems are also proposed. Finally, different bioreactor options are explored and their advantages are analyzed.

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“…Several methods can be employed to overcome recalcitrance during cryopreservation. These include one-or two-step freezing protocols and the use of various cryoprotectants (to minimize ice crystal formation and cell damage) or modification of cryopreservation protocols, e.g., by using: the most effective but least toxic vitrification solutions; pre-culture treatment involving sugars, abscisic acid or proline; progressive osmotic dehydration at high sucrose concentrations; and increased cooling/warming rates [3][4][5][6][7]. Sometimes, these protocols are lengthy, and this restricts their use to small-scale cryopreservation of plants/cell lines.…”

Section: Introductionmentioning

confidence: 99%

“…Sometimes, these protocols are lengthy, and this restricts their use to small-scale cryopreservation of plants/cell lines. As a result, a much simpler method would be most welcome [6]. The effective cryopreservation of ferns has been described for the gametophytes of 18 species [5,[8][9][10] and the young sporophytes of a single species of epiphytic fern, namely Platycerium ridleyi H. Christ.…”

Section: Introductionmentioning

confidence: 99%

A simple way to overcome the recalcitrance of the water fern Ceratopteris thalictroides (L.) Brongn. to cryopreservation

2015

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Ceratopteris thalictroides is a water fern very sensitive to both dehydration and low temperature. This study focuses on the cryopreservation of this species by encapsulation-dehydration technique, in particular on the effects of pre-culture step, alginate bead size and the physical conditions of culture on the cryopreservation efficiency. Encapsulated and non-precultured gametophytes did not survive cooling with liquid nitrogen. When cryopreservation was preceded by a 2-week period of pre-culture, regrowth reached 42.1%. Reduction in the size of the alginate bead, and culture in total darkness resulted in improved gametophyte regrowth capacity (75.5% or 81.7%, respectively). The best results (91.3%) were obtained when all factors tested occurred simultaneously. The gametophytes recovered very quickly and sporophytes were formed within 4 weeks after rewarming. These simple improvements can be used, not only for the cryopreservation of gametophytes in cryptogams but also for some recalcitrant species of seed plants.

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High-Throughput Cryopreservation of Plant Cell Cultures for Functional Genomics

Cited by 40 publications

References 24 publications

Generation of Triple-Transgenic Forsythia Cell Cultures as a Platform for the Efficient, Stable, and Sustainable Production of Lignans

Generation of Triple-Transgenic Forsythia Cell Cultures as a Platform for the Efficient, Stable, and Sustainable Production of Lignans

Improving Pharmaceutical Protein Production in Oryza sativa

A simple way to overcome the recalcitrance of the water fern Ceratopteris thalictroides (L.) Brongn. to cryopreservation

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