Characterization of aggregate size in Taxus suspension cell culture

Kolewe, Martin E.; Henson, Michael A.; Roberts, Susan C.

doi:10.1007/s00299-010-0837-5

Cited by 31 publications

(29 citation statements)

References 22 publications

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“…intracellular + extracellular: both in aqueous and PFD phases) yield of paclitaxel was obtained in PFD-degassed carrying cultures after two weeks of elicitation. Under the conditions of the current study we also observed in most of the cases higher lignan contents after two week elicitation, however, the PFD-aerated supported elicited cultures seemed to be more favourable for lignan accumulation (Tables 3, 4) likely due to generated to a higher extent than in PFD-degassed supported cultures oxidative stress which is believed to affect plant secondary metabolism (Shilpa et al 2010;Kolewe et al 2010). PFD application in the function of in situ extrahent could also contribute to the lower metabolite feedback inhibition and diminished cytotoxic metabolites accumulation in aqueous phases of the medium which seemed to be often the reason of limited secondary metabolites production (Malik et al 2013;Kolewe et al 2010).…”

Section: Lignan Accumulation In Cultures Of Atma and Kt Hairy Root LImentioning

confidence: 64%

Lignan accumulation in two-phase cultures of Taxus x media hairy roots

Sykłowska-Baranek

Łysik

Jeziorek

et al. 2018

Plant Cell Tiss Organ Cult

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The biosynthetic potential for six lignans accumulation in two lines of Taxus x media hairy roots was investigated. The cultures of KT and ATMA hairy root lines were supplemented with precursors: coniferyl alcohol (CA 1, 10 or 100 µM) and/or l-phenylalanine (100 µM PHEN) and/or methyl jasmonate (100 µM MeJa). Moreover the two-phase in vitro cultures supported with perfluorodecalin (PFD) as a gas carrier and in situ extrahent were used. The hairy root lines differed in lignan production profiles. In the control untreated cultures KT roots did not accumulate secoisolariciresinol and lariciresinol while ATMA roots did not accumulate matairesinol. In ATMA roots the treatment with CA (1 or 10 µM) resulted in the production of lariciresinol and secoisolariciresinol whereas solely lariciresinol was present after 100 µM CA application. Elicitation with 1 µM CA and MeJa yielded with hydroxymatairesinol aglyca and lariciresinol glucosides with their highest content 37.88 and 3.19 µg/g DW, respectively. The stimulatory effect of simultaneous treatment with 1 µM CA, PHEN and MeJa on lignan production was observed when the cultures were supplemented with PFD-aerated or degassed. In ATMA root cultures these applied conditions were the most favourable for matairesinol content which amounted to 199.86 and 160.25 µg/g DW in PFD-aerated and PFD-degassed supported cultures, respectively. In KT root cultures solely, hydroxymatairesinol and coniferin/CA content was enhanced with their highest yield 59.29 and 134.60 µg/g DW in PFD-aerated and PFD-degassed cultures, respectively.

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Section: Lignan Accumulation In Cultures Of Atma and Kt Hairy Root LImentioning

confidence: 64%

Lignan accumulation in two-phase cultures of Taxus x media hairy roots

Sykłowska-Baranek

Łysik

Jeziorek

et al. 2018

Plant Cell Tiss Organ Cult

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“…A Multisizer 3™ Coulter counter equipped with a 2000 µm aperture (Beckman Coulter, Brea, CA, USA) was used to determine total biomass dry weight based on previously published correlations (Kolewe et al 2010). For analysis, two × 2 mL samples of well-mixed culture broth (cells plus media) were taken from each flask.…”

Section: Methodsmentioning

confidence: 99%

Methyl jasmonate represses growth and affects cell cycle progression in cultured Taxus cells

et al. 2014

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Methyl jasmonate (MeJA) elicitation is an effective strategy to induce and enhance synthesis of the anticancer agent paclitaxel (Taxol®) in Taxus cell suspension cultures; however, concurrent decreases in growth are often observed, which is problematic for large scale bioprocessing. Here, increased accumulation of paclitaxel in Taxus cuspidata suspension cultures with MeJA elicitation was accompanied by a concomitant decrease in cell growth, evident within the first three days post-elicitation. Both MeJA-elicited and mock-elicited cultures exhibited similar viability with no apoptosis up to day 16 and day 24 of the cell culture period, respectively, suggesting that growth repression is not attributable to cell death. Flow cytometric analyses demonstrated that MeJA perturbed cell cycle progression of asynchronously dividing Taxus cells. MeJA slowed down cell cycle progression, impaired the G1/S transition as observed by an increase in G0/G1 phase cells, and decreased the number of actively dividing cells. Through a combination of deep sequencing and gene expression analyses, the expression status of Taxus cell cycle-associated genes correlated with observations at the culture level. Results from this study provide valuable insight into the mechanisms governing MeJA perception and subsequent events leading to repression of Taxus cell growth.

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“…For elicitation, 200 μM methyl jasmonate (MeJA) was added on day 7 post-transfer during the mid-exponential phase of growth, as described previously [34]. A Multisizer 3 ™ Coulter counter equipped with a 2,000 μm aperture (Beckman Coulter, Brea, CA) was used to measure culture aggregate size distributions, as described previously [30]. As the total aggregate volume was previously shown to correlate directly with biomass [30], this measurement was also used to determine dry weight (DW), and all DW data presented here were based on this correlation.…”

Section: Methodsmentioning

confidence: 99%

“…In Taxus suspension cultures, aggregates ranging from less than 100 μm to well over 2 mm have been observed [30]. Cells within these aggregates are subject to different microenvironments, leading to cell-cell differences in morphology [31] and metabolism [32].…”

Section: Introductionmentioning

confidence: 99%

Contribution of taxane biosynthetic pathway gene expression to observed variability in paclitaxel accumulation in Taxus suspension cultures

Patil¹,

Kolewe²,

Normanly³

et al. 2012

Biotechnology Journal

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Variability in product accumulation is one of the major obstacles limiting the widespread commercialization of plant cell culture technology to supply natural product pharmaceuticals. Despite extensive process engineering efforts, which have led to increased yields, plant cells exhibit variability in productivity that is poorly understood. Elicitation of Taxus cultures with methyl jasmonate (MeJA) induces paclitaxel accumulation, but to varying extents in different cultures. In this work, cultures with different aggregation profiles were established to create predictable differences in paclitaxel accumulation upon MeJA elicitation. Expression of known paclitaxel biosynthetic genes in MeJA-elicited cultures exhibiting both substantial (15-fold) and moderate (2-fold) differences in paclitaxel accumulation was analyzed using qRT-PCR. Each population exhibited the characteristic large increase in paclitaxel pathway gene expression following MeJA elicitation; however, differences in expression between populations were minor, and only observed for the cultures with the 15-fold variation in paclitaxel content. These data suggest that although upregulation of biosynthetic pathway gene expression contributes to observed increases in paclitaxel synthesis upon elicitation with MeJA, there are additional factors that need to be uncovered before paclitaxel productivity can be fully optimized.

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Characterization of aggregate size in Taxus suspension cell culture

Cited by 31 publications

References 22 publications

Lignan accumulation in two-phase cultures of Taxus x media hairy roots

Lignan accumulation in two-phase cultures of Taxus x media hairy roots

Methyl jasmonate represses growth and affects cell cycle progression in cultured Taxus cells

Contribution of taxane biosynthetic pathway gene expression to observed variability in paclitaxel accumulation in Taxus suspension cultures

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