WO2005064002A1 - Method for mass production of secondary metabolites in plant cell culture by treatment of an alkanoic acid or salt thereof - Google Patents
Method for mass production of secondary metabolites in plant cell culture by treatment of an alkanoic acid or salt thereof Download PDFInfo
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- WO2005064002A1 WO2005064002A1 PCT/KR2004/003491 KR2004003491W WO2005064002A1 WO 2005064002 A1 WO2005064002 A1 WO 2005064002A1 KR 2004003491 W KR2004003491 W KR 2004003491W WO 2005064002 A1 WO2005064002 A1 WO 2005064002A1
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- C12P15/00—Preparation of compounds containing at least three condensed carbocyclic rings
Definitions
- This invention relates to a method for mass production of secondary
- metabolites in plant cell culture and more specifically, to a method for production of secondary metabolites by using plant cell culture, characterized in that a faster growth of plant cells and the enhanced productivity of secondary
- metabolites are achieved in plant cell culture by treating culture medium with an alkanoic acid or salt thereof.
- the culture environments such as temperature, lighting, pH of the medium,
- genes relating to defense mechanisms while at the same time repressing the expression of genes relating to cell cycle control such as p34cdc2 protein kinase and mitotic cyclin (Logemann et al., Plant Journal 8:865-876, 1995).
- An objective of the present invention is to provide a method for mass production of secondary metabolites in plant cell cultures. Another objective of the present invention is to provide optimal conditions in the treatment concentrations, time of treatment, and the number of repeated treatments of alkanoic acid or salt thereof to enhance the productivity of secondary metabolites in plant cell cultures.
- the present invention provides a method for production of secondary metabolites by plant cell culture which includes the step of culturing plant cells upon treatment of the culture
- the present invention provides a method for mass production of secondary metabolites from plant cells by using alkanoic acid or salt thereof
- metabolites of plant origin such as paclitaxel, corosolic acid and the like.
- Fig. 1 shows time course of changes in dry cell weight of Taxus
- chinensis cell line SYG-1 after treating with 0 to10 mM of sodium butyrate on
- Fig. 2 shows the production pattern of paclitaxel in Taxus chinensis
- FIG. 3 is a photograph showing an electrophoresis result of the
- Fig. 4 shows time course of changes in the change in the dry cell
- Taxus chinensis cell line SYG-1 after culture following treatment with
- Fig. 5 shows the production pattern of paclitaxel after treating the
- Fig. 6 shows the result of paclitaxel production from Taxus chinensis
- Fig. 7 shows taxane produced from Taxus chinensis cell line SYG-1
- Fig. 8 shows tome course of changes in dry cell weight of Taxus
- chinensis cell line SYG-1 after treating with sodium propionate.
- Fig. 9 shows the result of paclitaxel production from Taxus chinensis
- Fig. 10 shows the result of paclitaxel production from Taxus chinensis
- SF sodium acetate
- SP sodium propionate
- SB sodium butyrate
- FIG. 11 and 12 show HPLC charts of suspension culture solution of
- concentration of alkanoic acid or salt thereof enhances cell growth, and found the optimal conditions for treating with alkanoic acid or salt thereof to produce secondary metabolites in plant cell cultures in mass quantities.
- secondary metabolites There are a wide variety of secondary metabolites that can be
- Table 2 shows examples of the above secondary metabolites and plant cells that can be used in production thereof.
- the method in accordance with the present invention for mass production of secondary metabolites in plant cell culture can be applied to all plant cells that produce secondary metabolites.
- the method can enhance productivity of secondary metabolites by applysing it to various plant cells displaying low productivity of secondary metabolites, and in particular be used in commercial production of paclitaxel by applying to Taxus genus cells
- paclitaxel used to produce paclitaxel which is proven to be effective in treatment of treatment-resistant ovarian cancer and breast cancer.
- Taxus cells belonging to the Taxus genus can have enhanced productivity of secondary metabolites according to the
- Taxus genus includes, but is not limited
- Taxus bacata Taxus brevifolia
- Taxus canadensis Taxus chinensis
- Taxus chinensis Taxus
- Taxus flo dana cuspidata, Taxus flo dana, Taxus globosa, Taxus media, Taxus wallichiana,
- Taxus yunnanensis Mass production of paclitaxel and taxane from plant cells
- a method for mass production of secondary metabolites in plant cell cultures according to the present invention includes the step of treating the plant cell culture with at least one alkanoic acid or salt thereof. .
- the above plant cell culture As it is widely known in the related art, the above plant cell culture
- plant cell culture media can comprise nutrients and other factors necessary to maintain the viability of plant cells, that is, carbon sources, nitrogen sources, salts, vitamins and the like.
- the plant cell culture media of the present invention can be media widely used in culturing plant cells, for example, but not limited to
- B5 medium comprising casein hydrolysate (see:
- a plant cell culture medium according to the present invention comprises selectively factors that can induce the production of secondary metabolites.
- factors include plant hormones, biosynthetic precursors or elicitors and signal couplers of secondary metabolites and the like. These factors added in the medium stimulate the production of secondary metabolites.
- the preferred inducing agent is silver
- nitrate and is preferably present in the culturing medium in the concentration range between 1uM and 15uM and added to the medium in the early stages of
- culture methods and conditions can be selected among
- Alkanoic acid according to the present invention is a compound linked
- n can be an integer from 1 to 9, preferably from 3 to 6.
- an alkanoic acid can be an alkaline metal salt, for example, sodium (Na), potassium (K) and the like are suitable.
- salt of butyric acid or salt of propionic acid preferably sodium butyrate or sodium propionate can be used.
- Alkanoic acids or salts thereof play a role in controlling the plant cell cycle by inducing modification of chromosome structure in cells by increasing
- Alkanoic acid or salt thereof may be present in culture medium at a concentration of between 0.01 to 500 mM, preferably between 0.1 mM to 200 mM, and more preferably between 0.1 mM to 20 mM, but is most preferably to
- Taxus chinensis cell growth is enhanced on culturing
- paclitaxel is increased significantly to 1.97 times that of control (Fig. 2).
- the treatment time of alkanoic acid or salt thereof to culture medium can be from prior to inoculation of the culture medium with plant cells to the end of growth and activity of the cells, and preferably the early log growth phase of the cells. It is more preferable, however, to adjust the time of treatment with alkanoic acid or salt thereof depending on plant cell type.
- the medium may be
- alkanoic acid or salt thereof from day 0 to day 21 of culture, and more preferably from day 0 to day 14 of culture.
- Alkanoic acid or salt thereof induces physiological changes of plant cells, and particularly induces changes such as inhibition of histone deacetylase activity or suppression of cell cycle related gene expression.
- the alkanoic acid or salt thereof is present in the medium at a constant concentration. Therefore, after the initial treatment of the culture medium with alkanoic acid or salt thereof, the culture medium may be treated one or more times at regular intervals. And alkanoic acid or salt
- concentration of the alkanoic acid or salt thereof be varied having regard to the
- Taxus chinensis cells can be treated with alkanoic acid or
- a method of the present invention can be applied to increase the
- Type II diabetes by Eriobotrya japonica cell culture.
- the present invention provides plant cell culture media and media for the production of secondary metabolites from plant cell culture
- alkanoic acid or salt thereof may be any suitable alkanoic acid or salt thereof.
- the alkanoic acid or salt thereof may be any suitable alkanoic acid or salt thereof.
- the concentration of the alkanoic acid or salt thereof may be appropriately varied having regard to the
- EXAMPLE 1 The effect of treating plant cell cultures with sodium
- Taxus chinensis SYG-1 cell line (KCTC-0232BP) was used to produce paclitaxel and taxane compounds.
- butyrate was added at concentrations of 0, 0.5, 1 , 5 and 10 mM, respectively
- cell weight is weight of cells determined after drying in a drying oven at 60 ° C
- lane A is a size marker
- lane B is a non-treated sample
- lane C is a sample treated with 1 mM of
- sodium butyrate and lane D is a sample treated with 5 mM of sodium butyrate.
- EXAMPLE 2 Determination of time of sodium butyrate treatment Sodium butyrate was added at concentrations of 1 mM on day 0, day
- Fig. 4 shows the cell growth according to the treatment time of sodium
- FIG. 5 shows paclitaxel production (in the Fig. 4 and Fig. 5 - ⁇ :
- non-treated sample o: sample treated with 1 mM of sodium butyrate on day 0
- paclitaxel productivity was highest when 1 mM of sodium butyrate was treated
- EXAMPLE 3 Repetitive treatment of sodium butyrate While culturing Taxus chinensis SYG-1 cell by using the same
- Taxus chinensis SYG-1 cell While culturing Taxus chinensis SYG-1 cell by using the same method as in EXAMPLE 1-1 , 1 Mm of sodium butyrate was added on day 7 and day 14 of culture. The culture was sampled on day 28, day 36 and day 43 of culture in order to determine the productivity of taxane compounds.
- Fig. 7 shows the productivity of taxane compounds (rate of increase
- butyrate on secondary metabolite productivity increase is a kind of induction
- Taxus chinensis SYG-1 cells While culturing Taxus chinensis SYG-1 cells, 0.5 mM or 1 Mm of
- Fig. 8 shows the cell growth of SYG-1 cultured with sodium
- Fig. 9 shows the productivity of paclitaxel (in the Fig.
- sodium propionate was 1 mM and when treated two times repeatedly.
- Fig. 10 shows paclitaxel productivity of Taxus chinensis SYG-1 cells
- SA sodium propionate
- SB sodium butyrate
- VA valeric acid
- induced callus was transferred to agar-free liquid culture medium and suspension cultured at 24 °C, 120 rpm in the dark.
- the established suspension cultured cells of Eriobotrya japonica was subcultured in the above medium at two-week intervals.
- the suspension culture cell of Eriobotrya japonica was treated with
- Fig. 11 and 12 show HPLC charts of extracts from Eriobotrya japonica cells cultures in the absence(Fig. 11) and the presence(Fig. 12) of 0.5 mM of
Abstract
The present invention relates to a method for mass production of secondary metabolites in plant cell culture, more specifically, to a method for production of secondary metabolites comprising the step of culturing plant cells in a medium treated with alkanoic acid or salt thereof. The present invention can contribute to the commercial production of useful secondary metabolites by providing a method for mass production of secondary metabolites from plant cells.
Description
DESCRIPTION
METHOD FOR MASS PRODUCTION OF SECONDARY METABOLITES IN
PLANT CELL CULTURE BY TREATMENT OF AN ALKANOIC ACID OR
SALT THEREOF Technical Field
This invention relates to a method for mass production of secondary
metabolites in plant cell culture, and more specifically, to a method for production of secondary metabolites by using plant cell culture, characterized in that a faster growth of plant cells and the enhanced productivity of secondary
metabolites are achieved in plant cell culture by treating culture medium with an alkanoic acid or salt thereof.
Background Art Plants are a useful source for producing a wide variety of secondary
metabolites which are used as pharmaceuticals, pesticides, spices, pigments, food additives, cosmetics and the like (table 1). However, while the demands for secondary metabolites in various areas of industries are increasing, the supply of secondary metabolites produced by extraction from plants is limited.
Therefore there have been efforts to commercially mass-produce secondary metabolites of plant origin by using plant cell culturing techniques (Stockigt et al., Plant Cell Tissue Org. Cult. 43: 914-920, 1995).
Table 1
However, mass production of secondary metabolites through plant cell culture is still difficult due to problems such as instability of cultured cell lines, low productivity, slow growth, scale-up problems and the like. Various efforts have been made to try and overcome the low productivity in plant cell cultures, and they include the following methods: 1) adjustment of nutrient sources in the media such as addition of sugar, nitrate salts, phosphate salts, growth control agents and precursors; 2) optimization of
the culture environments such as temperature, lighting, pH of the medium,
shaking and aeration conditions; 3) treatment with elicitors to enhance productivity; 4) permeabilization of cell membranes and two-phase culture for effective recovery of secondary metabolites; 5) metabolic engineering which enhances productivity of secondary metabolites by modifying genes involved in
the biosynthesis of secondary metabolites or introduction of exogenous genes. However, these trials were only effective for particular plant cells or secondary metabolites, and a method that can generally be applied to most plant cell cultures and secondary metabolites has not yet been established.
In nature, plants produce secondary metabolites as a defense mechanism against attack by pathogens, and it has been reported that in some
plant cell cultures production of secondary metabolites is enhanced by elicitors
originated from pathogens (US. 5,019,504). These elicitors activate genes
relating to defense mechanisms while at the same time repressing the expression of genes relating to cell cycle control such as p34cdc2 protein kinase and mitotic cyclin (Logemann et al., Plant Journal 8:865-876, 1995).
Also it is known that the HC toxin produced by Cochliobolus carbonum, a pathogen of corn, represses the activity of histone deacetylase (Brosch et al.,
Plant Cell 7:1941-1950, 1995). On the other hand, butyric acid or sodium butyrate as inhibitors of histone deacetylase induces hyperacetylation of histones H3 and H4 (Riggs et al., Nature 263:462-464, 1977). It was also reported that increased acetylation of histones by butyric acid treatment induces modification of chromosome structure in cells to enhance activity in transcription and has an
effect on the change of cell differentiation states (Thome et al., Eur. J. Biochem. 193:701-713, 1990), and induces apoptosis in some cells (Bhatia et al., Cell Growth Diff. 6: 937-944, 1995). Based on the above range of physiological activity of butyric acid, some researchers have developed a method for enhancing the expression level of exogenous proteins by treating animal cell
culture media with butyric acid or sodium butyrate in order to increase transcription of exogenous genes and enhance expression of exogenous protein (US 6,228,618).
Despite the wide range of physiological activity of butyric acid, there
has not been much research on the activity and functional mechanism of
butyric acid on plant cell cultures, and only study of the effect of butyric acid on
growth of plant cells and differentiation of plant tissues or cells have been
carried out (Tramontano and Scanlon, Phytochernistry 41 :85-88, 1996).
Disclosure
Technical Problem An objective of the present invention is to provide a method for mass production of secondary metabolites in plant cell cultures. Another objective of the present invention is to provide optimal conditions in the treatment concentrations, time of treatment, and the number of repeated treatments of alkanoic acid or salt thereof to enhance the productivity of secondary metabolites in plant cell cultures.
Technical Solution In order to achieve the above objectives, the present invention provides a method for production of secondary metabolites by plant cell culture which includes the step of culturing plant cells upon treatment of the culture
medium with alkanoic acid or salt thereof, wherein the alkanoic acid or salt thereof increases the productivity of secondary metabolites by plant cells.
Advantageous Effects
The present invention provides a method for mass production of
secondary metabolites from plant cells by using alkanoic acid or salt thereof
which are substances capable of greatly increasing productivity of secondary
metabolites in plant cell cultures. By using the present invention, it is possible
to greatly increase the productivity of secondary metabolites of plant cells
which are known to have very low productivity. Therefore the present invention
can greatly benefit the production of commercially useful secondary
metabolites of plant origin, such as paclitaxel, corosolic acid and the like.
Description of Drawings
Fig. 1 shows time course of changes in dry cell weight of Taxus
chinensis cell line SYG-1 after treating with 0 to10 mM of sodium butyrate on
day 7 of culture.
Fig. 2 shows the production pattern of paclitaxel in Taxus chinensis
cell line SYG-1 after treating with 0 to10 mM of sodium butyrate on day 7 of
culture. Fig. 3 is a photograph showing an electrophoresis result of the
genomic DNA of Taxus chinensis cell line SYG-1 after culture following
treatment with 0, 1 and 5 mM of sodium butyrate respectively on day 7 of culture.
Fig. 4 shows time course of changes in the change in the dry cell
weight of Taxus chinensis cell line SYG-1 after culture following treatment with
1.0 mM of sodium butyrate on different days of culture. Fig. 5 shows the production pattern of paclitaxel after treating the
Taxus chinensis cell line SYG-1 with 1.0 mM of sodium butyrate at different
times. Fig. 6 shows the result of paclitaxel production from Taxus chinensis
cell line SYG-1 after treating with sodium butyrate at different number of
repeated treatments. Fig. 7 shows taxane produced from Taxus chinensis cell line SYG-1
after treating with sodium butyrate. Fig. 8 shows tome course of changes in dry cell weight of Taxus
chinensis cell line SYG-1 after treating with sodium propionate.
Fig. 9 shows the result of paclitaxel production from Taxus chinensis
cell line SYG-1 after treating with sodium propionate. Fig. 10 shows the result of paclitaxel production from Taxus chinensis
cell line SYG-1 after culturing in medium containing 1 mM of sodium formate
(SF), sodium acetate (SA), sodium propionate (SP), sodium butyrate (SB) or
valeric acid (VA) respectively. Fig. 11 and 12 show HPLC charts of suspension culture solution of
Eriobotrya japonica and suspension culture solution of Eriobotrya japonica
where 0.5 mM of sodium butyrate is added.
Mode for Invention
The inventors of the present invention have researched to provide an
effective method for enhancing productivity of secondary metabolites which
can be applied to various plant cell cultures, and have confirmed that treating the medium for plant cell culture with alkanoic acid or salt thereof can enhance productivity of secondary metabolites in plant cells.
The inventors have accomplished the present invention by
discovering that treating plant cell culture media with a relative high concentration of alkanoic acid or salt thereof significantly inhibits cell growth
and increases the productivity of secondary metabolites, while an appropriate
concentration of alkanoic acid or salt thereof enhances cell growth, and found the optimal conditions for treating with alkanoic acid or salt thereof to produce secondary metabolites in plant cell cultures in mass quantities. There are a wide variety of secondary metabolites that can be
produced from plants, and there a range of different techniques applied according to characteristics of plant species and secondary metabolites produced from them. Table 2 shows examples of the above secondary metabolites and plant cells that can be used in production thereof.
Table 2
The method in accordance with the present invention for mass production of secondary metabolites in plant cell culture can be applied to all plant cells that produce secondary metabolites. Preferably, the method can enhance productivity of secondary metabolites by applysing it to various plant cells displaying low productivity of secondary metabolites, and in particular be used in commercial production of paclitaxel by applying to Taxus genus cells
used to produce paclitaxel which is proven to be effective in treatment of treatment-resistant ovarian cancer and breast cancer.
That is, various species of Taxus cells belonging to the Taxus genus can have enhanced productivity of secondary metabolites according to the
method in the present invention for mass production of secondary metabolites
in plant cell cultures. Examples of the Taxus genus includes, but is not limited
to, Taxus bacata, Taxus brevifolia, Taxus canadensis, Taxus chinensis, Taxus
cuspidata, Taxus flo dana, Taxus globosa, Taxus media, Taxus wallichiana,
Taxus yunnanensis. Mass production of paclitaxel and taxane from plant cells
of Taxus genus can be possible with the method. Specifically, a method for mass production of secondary metabolites in plant cell cultures according to the present invention includes the step of treating the plant cell culture with at least one alkanoic acid or salt thereof. . As it is widely known in the related art, the above plant cell culture
media can comprise nutrients and other factors necessary to maintain the viability of plant cells, that is, carbon sources, nitrogen sources, salts, vitamins and the like. Also, the plant cell culture media of the present invention can be media widely used in culturing plant cells, for example, but not limited to
Murashige & Skoog medium, Gamborg B5 medium, Linsmaier & Skoog
medium, which can also be used with various additives on occasion or with some components removed. For example, in case of producing paclitaxel and taxane compounds by culturing Taxus chinensis, B5 medium comprising casein hydrolysate (see:
Gamborg et al., Can. J. Biochem., 45 : 417-421(1968)) or a modified Gamborg B5 medium, with 60 g/L of sucrose added to the said B5 medium can be used, and its composition is shown in Table 3 as below. (See: Korean Patent No. 0266448)
Table 3
In addition, a plant cell culture medium according to the present invention comprises selectively factors that can induce the production of secondary metabolites. Such factors include plant hormones, biosynthetic precursors or elicitors and signal couplers of secondary metabolites and the like. These factors added in the medium stimulate the production of secondary
metabolites in plant cells through various routes and can induce a synergetic effect on the productivity of secondary metabolites together with the treatment with alkanoic acid or salt thereof according to the present invention.
For example, in the case of producing paclitaxel and taxane compounds by culturing Taxus chinensis, the preferred inducing agent is silver
nitrate and is preferably present in the culturing medium in the concentration
range between 1uM and 15uM and added to the medium in the early stages of
culture. In addition, culture methods and conditions can be selected among
known methods based on plant cell types or secondary metabolites. Alkanoic acid according to the present invention is a compound linked
in a single chain having a carbonyl group at one end, and shown as CnH2nO2.
The above n can be an integer from 1 to 9, preferably from 3 to 6. The salt of
an alkanoic acid can be an alkaline metal salt, for example, sodium (Na), potassium (K) and the like are suitable. In case of producing paclitaxel and taxane compounds by culturing Taxus chinensis, salt of butyric acid or salt of propionic acid, preferably sodium butyrate or sodium propionate can be used. Alkanoic acids or salts thereof play a role in controlling the plant cell cycle by inducing modification of chromosome structure in cells by increasing
the acetylation of histones. Particularly, cessation of cell growth is observed during cell culture of Taxus chinensis cell culture is treated with sodium
butyrate above a certain concentration (Fig. 1), DNA bands that are multiples of a certain length in size appear on electrophoresis of genomic DNA of cells treated with 5 mM of sodium butyrate, which is characteristic of apoptosis (Fig.
3). The above results indicate that modification of chromosome structure in Taxus chinensis cells was induced by sodium butyrate and that this lead to cessation of cell growth and apoptosis.
Alkanoic acid or salt thereof may be present in culture medium at a concentration of between 0.01 to 500 mM, preferably between 0.1 mM to 200
mM, and more preferably between 0.1 mM to 20 mM, but is most preferably to
adjust the concentration to suit the particular plant cell type. Taxus chinensis
may be cultured in a medium containing alkanoic acid or salt thereof at a
concentration of between 0.5 mM and 10 mM, and preferably between 0.7 mM and 1.5 mM. Particularly, Taxus chinensis cell growth is enhanced on culturing
in a medium containing 1 mM of sodium butyrate (Fig. 1), and the productivity
of paclitaxel is increased significantly to 1.97 times that of control (Fig. 2).
The treatment time of alkanoic acid or salt thereof to culture medium can be from prior to inoculation of the culture medium with plant cells to the end of growth and activity of the cells, and preferably the early log growth phase of the cells. It is more preferable, however, to adjust the time of treatment with alkanoic acid or salt thereof depending on plant cell type. For example, in the case of Taxus chinensis cell culture, the medium may be
treated with alkanoic acid or salt thereof from day 0 to day 21 of culture, and more preferably from day 0 to day 14 of culture. Alkanoic acid or salt thereof induces physiological changes of plant cells, and particularly induces changes such as inhibition of histone deacetylase activity or suppression of cell cycle related gene expression. The
above changes are reversible; therefore the changed characteristics of the cells return to its original state when the alkanoic acid or salt thereof is depleted. So, it is preferable that the alkanoic acid or salt thereof is present in the medium at a constant concentration. Therefore, after the initial treatment of the culture medium with alkanoic acid or salt thereof, the culture medium
may be treated one or more times at regular intervals. And alkanoic acid or salt
thereof may be maintained in the medium at a concentration of between 0.01
and 500 mM, preferably between 0.1 mM and 200 mM, and more preferably
between 0.2 mM and 20 mM. It is most preferable, however, that the
concentration of the alkanoic acid or salt thereof be varied having regard to the
particular plant cells. Taxus chinensis cells can be treated with alkanoic acid or
salt thereof in the medium one to three times during culture, and preferably two
to three times.
All appropriate plant cell culture methods known to the relevant field
of technology may be used in the cell culture of the present invention. For
example, batch culture, continuous culture, fed-batch culture, semi-continuous
batch process, immobilized culture, two-phase culture and the like may be
used and selected depending on plant cell type and characteristics of the
secondary metabolites. In one embodiment of the present invention, paclitaxel and taxane
compounds were produced by culturing Taxus chinensis cells according to the
present invention. As a result, the productivity of paclitaxel was increased six¬
fold and the productivity of taxane compounds was increased from about 1.6-
fold to about 9-fold depending on the taxane compound. A method of the present invention can be applied to increase the
productivity of corosolic acid, which can be used to treat anti-insulin-
independent (Type II) diabetes, by Eriobotrya japonica cell culture.
Also, the present invention provides plant cell culture media and
media for the production of secondary metabolites from plant cell culture
containing alkanoic acid or salt thereof. The alkanoic acid or salt thereof may
be present in the medium at a concentration of between 0.01 mM and 500 mM, preferably between 0.1 mM and 200 mM, more preferably between 0.1 mM and 20 mM. It is most preferable, however, that the concentration of the alkanoic acid or salt thereof may be appropriately varied having regard to the
particular plant cells. The present invention is further illustrated in the following examples, which should not be taken to limit the scope of the invention.
EXAMPLE 1 : The effect of treating plant cell cultures with sodium
butyrate
1-1. Determination of plant cell growth and productivity of secondary metabolites Taxus chinensis SYG-1 cell line (KCTC-0232BP) was used to produce paclitaxel and taxane compounds.
50 mi of SYG-1 culture solution incubated in a medium containing 30
g/L of sucrose (Korean patent NO.266448) for 14 days were inoculated to 50
ml of medium containing 60 g/L of sucrose in 250 mi Erlenmeyer flasks and
incubated in the dark at 24°C, 150 rpm for 14 days. Then, the cultures were
incubated at an elevated temperature of 29 °C for 28 days. Also, sodium
butyrate was added at concentrations of 0, 0.5, 1 , 5 and 10 mM, respectively
on day 7 of culture in order to increase paclitaxel productivity of SYG-1 , and
each culture was sampled on days 14, 21 , 28, 35, 42 of culture to measure cell
growth and paclitaxel productivity. Cell growth was observed by determining dry cell weight (DCW). Dry
cell weight is weight of cells determined after drying in a drying oven at 60 °C
for 24 hours following filtration of the sample from plant cell culture through Whatman No. 4 filter paper using a Buchner funnel. Paclitaxel productivity was measured by a quantitative analysis
method for paclitaxel and taxane compounds widely known to the relevant field of technology (Korean Patent No. 0266448). Cell growth and paclitaxel productivity of SYG-1 culture treated with
sodium butyrate was shown in Fig. 1 and Fig. 2 (Fig. 1 and Fig. 2 - D: not
treated, O: 0.5 mM sodium butyrate, Δ: 1.0 mM sodium butyrate, O: 5.0 mM
sodium butyrate, X: 10.0 mM sodium butyrate). When treated with 0.5 mM of sodium butyrate, there are no significant changes in cell growth and paclitaxel productivity. However, when treated with 1 mM of sodium butyrate, cell growth was greatly increased from the 14th day
of culture, and reached a peak of 23.22 g/L on day 28 and then gradually decreased. When treated with 5 mM and 10 mM of sodium butyrate, cell growth did not occur and the color of cells turned dark brown as apoptosis occurred. And on treating with 1mM of sodium butyrate, the quantity of paclitaxel produced was at a maximum of 133.8 mg/L on day 35 of culture, which is 1.97 times that of the control.
1-2. Determination of intracellular changes
Genomic DNA of 1 g (fresh weight) of Taxus chinensis SYG-1 cell
cultured in medium treated with 0 mM, 1 mM and 5 mM of sodium butyrate was
extracted by using a DNA extracting kit (DNeasy Plant Mini Kit, QIAGEN,
U.S.A.). 250 ug of the extracted genomic DNA was separated by
electrophoresis on an agarose gel (Fig. 3). In Fig. 3, lane A is a size marker,
lane B is a non-treated sample, lane C is a sample treated with 1 mM of
sodium butyrate and lane D is a sample treated with 5 mM of sodium butyrate.
Under the condition of treatment with 5 mM of sodium butyrate,
cessation of cell growth was confirmed (Fig. 1 ) and DNA bands that are
multiples of a certain length in size could be seen in the electrophoresis of
genomic DNA, which is characteristic of apoptosis. So, we could see that
sodium butyrate in the medium induced modification of chromosome structure
in Taxus chinensis cells which caused cessation of cell growth and apoptosis. EXAMPLE 2: Determination of time of sodium butyrate treatment Sodium butyrate was added at concentrations of 1 mM on day 0, day
7, day 14 and day 21 of culture respectively in Taxus chinensis SYG-1 was
cultured and a sample of each was removed from the culture on days 14, 21 ,
28, 35, 42 respectively, and cell growth and productivity of paclitaxel was
determined in the same method as in EXAMPLE 1. Fig. 4 shows the cell growth according to the treatment time of sodium
butyrate and Fig. 5 shows paclitaxel production (in the Fig. 4 and Fig. 5 - α:
non-treated sample, o: sample treated with 1 mM of sodium butyrate on day 0
of culture, Δ: sample treated with 1 mM of sodium butyrate on day 7 of culture,
O: sample treated with 1 mM of sodium butyrate on day 14 of culture, X:
sample treated with 1 mM of sodium butyrate on day 21 of culture). In case of Taxus chinensis SYG-1 treated with 1 mM of sodium butyrate, high cell growth was observed regardless of time of treatment with sodium butyrate in comparison with the non-treated control. Furthermore,
paclitaxel productivity was highest when 1 mM of sodium butyrate was treated
on day 7 of culture. On the basis of results in Fig. 4, the maximum specific growth rate of cell growth of Taxus chinensis SYG-1 depending on the time of treatment with 1 mM of sodium butyrate, was obtained and shown in Table 4. The earlier the time of treatment with sodium butyrate, the higher the maximum specific growth rate of cells, and maximum dry cell weight was attained sooner. However, maximum dry cell weight was highest being 23.22 mg/L, when 1 mM of sodium butyrate was treated on day 7 of culture. Table 4
EXAMPLE 3: Repetitive treatment of sodium butyrate While culturing Taxus chinensis SYG-1 cell by using the same
method as the EXAMPLE 1-1, 1 mM of sodium butyrate was added on day 1 and day 15 of culture, and then same concentration of sodium butyrate was
added up to three more times at 7-day intervals. Productivity of paclitaxel on
day 30 and day 37 of culture were determined (Fig. 6 - D: day 30 of culture,
0: day 37 of culture)
As a result, productivity of paclitaxel was increased in proportion to
the number of treatments. When 1 mM of sodium butyrate was repeatedly treated three more times, productivity of paclitaxel was 6.43 times higher
compared with control on day 37 of culture. And in case of treating with 1 mM of sodium butyrate on day 15 of culture followed by three repeated treatments,
the productivity of paclitaxel, was 4.95 times higher compared with the highest productivity attained with only two repeated treatments, as control.
EXAMPLE 4: Production of taxane compounds by treatment of
sodium butyrate
While culturing Taxus chinensis SYG-1 cell by using the same method as in EXAMPLE 1-1 , 1 Mm of sodium butyrate was added on day 7 and day 14 of culture. The culture was sampled on day 28, day 36 and day 43 of culture in order to determine the productivity of taxane compounds.
Fig. 7 shows the productivity of taxane compounds (rate of increase
or decrease of taxane compounds compared with control calculated as %);
D-cultured for 28 days, 0-cultured for 36 days, B-cultured for 43 days, A is
Bad II, B is 10-DAT, C is taxcultine, D is cephalomammine, E is 13-deacetyl taxchinin I, F is paclitaxel, G is benzyl analog, and H is H4. In Fig. 7, the productivity of all the taxane compounds was increased
significantly upon treatment with sodium butyrate, and particularly when
cultured for 28 days it increased greatly from about 1.6 to 9 times. However,
the degree of increase became smaller, being 1 to 3 times on day 36 of culture,
and became even smaller on day 43. This indicates that the effect of sodium
butyrate on secondary metabolite productivity increase is a kind of induction
effect, and is not continuous. That is, sodium butyrate induces production of
secondary metabolites for a period of time after treatment, but there is a
tendency to return to the original state. Furthermore, it can be seen that the
phenomenon of productivity increase is not limited to paclitaxel, but generally
applies to all secondary metabolites. EXAMPLE 5: Treatment of sodium propionate
While culturing Taxus chinensis SYG-1 cells, 0.5 mM or 1 Mm of
sodium propionate was treated on day 7 and day 14 of culture.
Fig. 8 shows the cell growth of SYG-1 cultured with sodium
propionate treatment and Fig. 9 shows the productivity of paclitaxel (in the Fig.
8 and Fig. 9 - D ' non-treated sample, O: sample treated with 0.5 mM of
sodium propionate on day 7 of culture, Δ: sample treated with 0.5 mM of
sodium propionate on day 7 and day 14 of culture, •: sample treated with 1
mM of sodium propionate on day 7 of culture, A : sample treated with 1 mM of
sodium propionate on day 7 and day 14 of culture). When treated with sodium propionate, cell growth of Taxus chinensis
SYG-1 cell was increased, and cell growth was rapid when the concentration of
sodium propionate was 1 mM and when treated two times repeatedly.
The higher the concentration of sodium propionate was and the
higher the number of treatments, the higher the productivity of paclitaxel was.
From the above results, it can be seen that alkanoic acid or salt
thereof other than sodium propionate can also increase the productivity of secondary metabolites in plant cell culture. EXAMPLE 6: Effect of various alkanoic acids
In culturing Taxus chinensis SYG-1 cells, 1 mM of sodium formate
(C1), sodium acetate (C2), sodium propionate (C3), sodium butyrate (C4) and valeric acid (C5) was added respectively on day 7 of culture. Fig. 10 shows paclitaxel productivity of Taxus chinensis SYG-1 cells
cultured in the medium including 1 mM of sodium formate (SF), sodium acetate
(SA), sodium propionate (SP), sodium butyrate (SB) or valeric acid (VA)
respectively. Salts of alkanoic acids containing one to five carbon atoms augmented paclitaxel productivity. EXAMPLE 7: Production of corosolic acid Callus and suspension culture was induced from Eriobotrya japonica,
a plant indigenous to Wando, Jeollanam-do province.
Collected leaves were treated with 70% alcohol for 60 seconds, with 1% sodium hypochlorite for 20 minutes, and then surface sterilized by washing three times with sterilized distilled water. Thereafter, the leaves were incubated in the dark at 24 °C in the culture medium of EXAMPLE 1-1 containing 0.7%
agar. After 3-4 weeks of culture, induced callus was transferred to agar-free liquid culture medium and suspension cultured at 24 °C, 120 rpm in the dark.
The established suspension cultured cells of Eriobotrya japonica was
subcultured in the above medium at two-week intervals.
The suspension culture cell of Eriobotrya japonica was treated with
0.5 mM of sodium butyrate followed by 14 days of culture, then corosolic acid production was confirmed. The method of extracting corosolic acid was carried out according to the quantitative analysis method for paclitaxel and
taxane compounds in EXAMPLE 1-1 , and detection of corosolic acid was
carried out by determining absorbance at 210 mM wavelength in flow of 40-80% acetonitrile solution at 1 ml/min flow rate. Fig. 11 and 12 show HPLC charts of extracts from Eriobotrya japonica cells cultures in the absence(Fig. 11) and the presence(Fig. 12) of 0.5 mM of
sodium butyrate, respectively. A corosolic acid peak was detected at 20.1 minutes of retention time. The productivity of corosolic acid was increased 63% on treatment with 0.5 mM of sodium butyrate.
Claims
1. A method for production of secondary metabolites in plant cell culture,
comprising the step of culturing plant cells by treating a culture medium with alkanoic acid or salt thereof represented as general formula (1) as follows, wherein the alkanoic acid or salt thereof increases the productivity of
secondary metabolites of plant cells.
(general formula 1 )
CnH2n02 Wherein, n is integer from 1 to 9.
2. The method according to claim 1 , wherein the plant cells are originated
from the Taxus genus or Eriobotrya japonica.
3. The method according to claim 2, wherein the Taxus genus is selected
from the group consisting of Taxus bacata, Taxus brevifolia, Taxus canadensis, Taxus chinensis, Taxus cuspidate, Taxus floridana, Taxus globosa, Taxus
media, Taxus wallichiana and Taxus yunnanensis.
4. The method according to claim 1, wherein the secondary metabolite is paclitaxel, a taxane compound or corosolic acid.
5. The method according to claim 1, wherein the alkanoic acid is propionic acid or butyric acid.
6. The method according to claim 1 , wherein the salt of alkanoic acid is alkaline metal salt of alkanoic acid.
7. The method according to claim 1 , wherein the culture medium is
treated with alkanoic acid or salt thereof at a concentration of between 0.1 mM
to 20 mM.
8. The method according to claim 1 , wherein the culture medium is
treated with alkanoic acid or salt thereof during the period between day 0 and
day 21 of culture.
9. The method according to claim 1 , wherein the alkanoic acid or salt
thereof is repeatedly treated one to five times.
10. A medium for producing secondary metabolites in plant cell culture
comprising plant cell culture medium and 0.1 mM to 20 mM of alkanoic acid or
salt thereof represented as general formula (1 ) as follows: (general formula 1 ) 
Wherein, n is integer from 1 to 9.
11. The medium according to claim 10, wherein the plant is selected from
the group consisting of Taxus bacata, Taxus brevifolia, Taxus canadensis,
Taxus chinensis, Taxus cuspidata, Taxus floridana, Taxus globosa, Taxus
media, Taxus wallichiana, Taxus yunnanensis and Eriobotrya japonica.
12. The medium according to claim 10, wherein the secondary metabolite is paclitaxel, a taxane compound or corosolic acid.
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| EP04808620A EP1709185A1 (en) | 2003-12-31 | 2004-12-29 | Method for mass production of secondary metabolites in plant cell culture by treatment of an alkanoic acid or salt thereof |
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| KR10-2004-0109149 | 2004-12-21 | ||
| KR1020040109149A KR100577094B1 (en) | 2003-12-31 | 2004-12-21 | Method for mass production of secondary metabolites in plant cell culture by treatment of an alkanoic acid or salt thereof |
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Cited By (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2007004827A1 (en) * | 2005-06-30 | 2007-01-11 | Samyang Genex Corporation | The method for production of corosolic acid in suspension culture of plant cells |
Citations (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO1987005626A1 (en) * | 1986-03-14 | 1987-09-24 | Celltech Limited | Production of proteins by cell culture |
| WO1989006686A1 (en) * | 1988-01-13 | 1989-07-27 | The Upjohn Company | Enhanced production of cellular proteins using butyrate |
| WO1996039488A1 (en) * | 1995-06-06 | 1996-12-12 | Genentech, Inc. | Process for controlling sialylation of proteins produced by mammalian cell culture |
| KR19980039738A (en) * | 1996-11-28 | 1998-08-17 | 손경식 | New Cell Culture Media for Glycation and Productivity of Mammalian Cell-Derived Glycoproteins |
-
2004
- 2004-12-29 EP EP04808620A patent/EP1709185A1/en not_active Withdrawn
- 2004-12-29 WO PCT/KR2004/003491 patent/WO2005064002A1/en not_active Application Discontinuation
Patent Citations (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO1987005626A1 (en) * | 1986-03-14 | 1987-09-24 | Celltech Limited | Production of proteins by cell culture |
| WO1989006686A1 (en) * | 1988-01-13 | 1989-07-27 | The Upjohn Company | Enhanced production of cellular proteins using butyrate |
| WO1996039488A1 (en) * | 1995-06-06 | 1996-12-12 | Genentech, Inc. | Process for controlling sialylation of proteins produced by mammalian cell culture |
| KR19980039738A (en) * | 1996-11-28 | 1998-08-17 | 손경식 | New Cell Culture Media for Glycation and Productivity of Mammalian Cell-Derived Glycoproteins |
Non-Patent Citations (1)
| Title |
|---|
| CHUA Y.L. ET AL: "The Transcriptional Enhancer of the Pea Plastocyanin Gene Associates with the Nuclear Matrix and Regulate Gene Expression through Histone Acetylation", THE PLANT CELL, vol. 15, June 2003 (2003-06-01), pages 1468 - 1479 * |
Cited By (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2007004827A1 (en) * | 2005-06-30 | 2007-01-11 | Samyang Genex Corporation | The method for production of corosolic acid in suspension culture of plant cells |
| US8101411B2 (en) | 2005-06-30 | 2012-01-24 | Samyang Genex Corporation | Method for production of corosolic acid in suspension culture of plant cells |
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