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12TH INTERNATIONAL CONFERENCE FUNCTIONAL FOOD INGREDIENTS AND NUTRACEUTICALS IN CHRONIC DISEASE: SCIENCE AND PRACTICE NOVEMBER 29-DECEMBER2 DALLAS, TX, USA
Teresa Serra, PhD
Researcher
Nutraceuticals & Controlled Delivery Unit - IBET/ITQB-UNL
e-mail: [email protected]
is the second most fatal and the third most diagnosed type of cancer worldwide
From 1981 to 2002…
Almost 74% of all drugs approved for cancer therapy were:
(i) natural products
(ii) based on natural products or
(iii) mimicked natural products in one form or another
In 2008: 7.5 million people died from cancer worldwide In 2020: it is estimated that mortality from cancer will increase to more than 10 million
Emerging interest in chemotherapeutic application of
Reverting chemoresistance
Phytochemicals (polyphenols and terpenes)
Anticancer effect
Inhibition of tumour cell mediated
protease activity
Attenuation of tumour angiogenesis Induction of cell cycle
arrest
Induction of apoptosis
…..
Evaluation of the antiproliferative effect and cell cycle modulation of several plant derived natural extracts in human colorectal cancer cells
Correlation of the bioactive effect with phytochemical composition of samples
SWEET CHERRIES OLIVES CACTUS PEAR CORK
• Crop residues Cherry culls (fruit that is not suitable to sell for eating due to small size and weight)
• Olive oil by-products (olive mill semi solid residue)
• Leaves
• Juice prodution residues (peels and seeds)
• Cork industry by-products
Bioactive rich fractions (e.g. polyphenols, carotenoids,
phytosterols, terpenes,...)
Reduces or eliminates the use or generation of
hazardous substances
Green sustainable processes
High pressure and
supercritical fluid
technology
Membrane Filtration
Adsorption process (with macroporous
resins)
Conventional Extraction
(with biocompatible
solvents)
• Total polyphenols content
• Total flavonoids content
• Total phenolic acids content
• Total procyanidin content
Spectrophotometric assays
• Total anthocyanin content
• Total betalain content
• Analysis of carotenoids
• TLC
• UPLC
•HPLC-DAD-FD-ED
•HPLC-MS/MS
• GC-MS
Chromatographic techniques
HT29 cells (Human colon adenocarcinoma)
ANTIPROLIFERATIVE EFFECT
CELL CYCLE ARREST
• Dose-response curves • Effective dose values (ED50)
MTT and MTS assays
by Flow Cytometry
Saco cherry culls
Perillyl alcohol
Chemoprevention of Colon Carcinogenesis by Dietary Perillyl Alcohol Reddy et al., 1997
Chemotherapy of pancreatic cancer with the monoterpene perillyl alcohol Stark et al., 1995
Perillyl Alcohol Inhibits Human Breast Cancer Cell Growth in vitro and in vivo Yuri et al., 2004
Effects of Perillyl alcohol on Melanoma in the Tpras Mouse Model Lluria-Prevatt et al., 2002
High Pressure Extraction with CO2 and ethanol
Higher selectivity
Short extraction times
GRAS solvents
Supercritical CO2 has been shown to be efficient in the extraction of perillyl alcohol from natural sources
SWEET CHERRIES NATURAL EXTRACTS
SFE (Supercritical Fluid Extraction)
CO2; P= 25 MPa;
T= 50ºC; t= 60 min
ESE (Enhanced Solvent Extraction)
CO2+EtOH (10-100%v/v)
P= 25 MPa; T= 50ºC;
t= 90 min
Dried cherry
1st step
2nd step
Methodology:
Fractioned High Pressure Extraction
10% EtOH
20% EtOH
40% EtOH
60% EtOH
75% EtOH
100% EtOH
To remove unwanted compounds
SWEET CHERRIES NATURAL EXTRACTS
0
20
40
60
80
100
120
A B C D E F G
Cel
l via
bilit
y (%
of c
ontro
l)
24h 48h 72h 96h
10% EtOH
20% EtOH
40% EtOH
60% EtOH
75% EtOH
100% EtOH
CO2
Tested concentration: 0.5mg/mL 24h 48h 72h 96h
Control
10% EtOH
20% EtOH
100m
Only two extracts (10%EtOH and 20%EtOH) inhibited cancer cell growth in a time
dependent manner and this effect is related with the presence of Perillyl Alcohol
• Antiproliferative effect
Serra et al. (2011), J Supercr Fluids,55, 184-191
The extract obtained with 10% EtOH exhibited the highest antiproliferative effect
(ED50=0.20 mg/mL) being 150 times more effective than fresh fruit
SWEET CHERRIES NATURAL EXTRACTS
Cherry extracts (0.5mg/mL) Doxorubicin (125nM) 10%EtOH
• Induction of cell cycle arrest
0
20
40
60
80
100
Control 4h 24h 48h 72h 96h
cell (
%)
G1 S G2/M
0
20
40
60
80
100
Control 4h 24h 48h 72h 96h
cell (
%)
G1 S G2/M
Cherry extracts induced cell cycle arrest in a different cell cycle checkpoint than doxorrubicin suggesting that they can be used in combination with the drug in chemotherapy
Cell cycle arrest in G1 Cell cycle arrest in G2/M
Serra et al. (2011), J Supercr Fluids, 55, 1007-1013
20%EtOH
0
20
40
60
80
100
Control 4h 24h 48h 72h 96h
cell (
%)
G1 S G2/M
SWEET CHERRIES NATURAL EXTRACTS
some studies showed that potent inhibition of tumour survival is achieved when combining drugs
with different cell cycle checkpoints
Cherry extracts (0.5mg/mL) 10%EtOH
• Induction of cell cycle arrest
0
20
40
60
80
100
Control 4h 24h 48h 72h 96h
cell (
%)
G1 S G2/M
Cell cycle modulation of cherry extracts was related with the presence of perillyl alcohol
Cell cycle arrest in G1 20%EtOH
0
20
40
60
80
100
Control 4h 24h 48h 72h 96h
cell (
%)
G1 S G2/M
0
20
40
60
80
100
Control 24h
cell
(%)
G1 S G2/M
Cell cycle arrest in G1
Perillyl alcohol (130 µg/mL)
SWEET CHERRIES NATURAL EXTRACTS
1
2 3
4
OLIVE - BASED NATURAL EXTRACTS
Membrane separation process
Conventional solvent extracton
C=220mg/g extract (dw)
EP1910257, 2008.
Olive natural extract derived from olive oil by-products is rich hydroxytyrosol – it contained 22% w/w of HT Matias, AA (2009), PhD thesis
Olive oil by-products
(olive mill semi solid residue)
Dried leaves
1- Hydroxytyrosol HT rich extract
2- Tyrosol 3- Caffeic acid 4- p-coumaric acid
2- Oleuropein
LT+OL rich
extract
Olive natural extract derived from dried leaves contains mainly luteolin derivatives and oleuropein
1- Luteolin derivatives
Ext. Folhas Oliveira Arbasana MS Scan25-Nov-201216:59:34
Time10.00 20.00 30.00 40.00 50.00 60.00 70.00 80.00 90.00 100.00 110.00 120.00
AU
0.0
2.5e-2
5.0e-2
7.5e-2
1.0e-1
1.25e-1
1.5e-1
1.75e-1
2.0e-1
2.25e-1
2.5e-1
2.75e-1
3.0e-1
3.25e-1
3.5e-1
3.75e-1
4.0e-1
4.25e-1
IBET_23Novembro012_24 2: Diode Array 280
Range: 4.704e-18.50
88.68
85.45
79.57
59.7392.53 106.61
1 1
1
1 2
OLIVE - BASED NATURAL EXTRACTS
• Antiproliferative effect
Matias, AA (2009), PhD thesis
HT rich extract - HT-rich extract
- Standard
Note: Cells were incubated with extract/compound for 4h and cell proliferation was evatuated after 24h
Olive HT-rich extract was more effective in inhibiting
cancer cell growth and inducing cell cycle arrest in the G1
phase than standard compound
• Cell cycle arrest
HT rich extract- C=25M (HT)
Hydroxytyrosol - C=100 M
OLIVE - BASED NATURAL EXTRACTS
• Antiproliferative effect
Note: Cells were incubated with extract/compound for 24h
LT+OL rich
extract
Oleuropein induced cell cycle arrest of HT29 cells in S phase
Oleuropein C=50 M
LT+OL rich extract
• Cell cycle arrest
LT+OL rich extract induced cell cycle arrest in both S and G2 phases
Luteolin was shown to induce cell cycle arrest in G2/M phase (Lim et al., 2006)
OPUNTIA - BASED NATURAL EXTRACTS
Hidroalcoholic extraction
Pressurized liquid extracton
Opuntia rubusta extract contains betalains pigments whereas Opuntia ficus indica extract present flavonoids (isorhamnetin and quercetin glycosides), terpenes and fatty acids (palmitic acid, octadecadienoic acid)
Opuntia rubusta fruit juice residues (seeds and peels)
Opuntia ficus indica fruit juice residues (seeds and peels)
Minutes
15.0 17.5 20.0 22.5 25.0 27.5 30.0 32.5 35.0 37.5 40.0 42.5 45.0 47.5 50.0 52.5 55.0 57.5
mAU
0
250
500
750
1000
1250
1500
1750
2000
2250
mAU
0
250
500
750
1000
1250
1500
1750
2000
2250
Detector 1-Scan-535 nm
Betalains
HPLC-DAD-UV 535nm
60% CO2: 40%EtOH v/v P= 20MPa; T= 313K
50% H2O :50%EtOH v/v
Minutes10 20 30 40 50 60 70 80 90 100 110
mAU
0
100
200
300
400
500
600
700
800
900
1000
mAU
0
100
200
300
400
500
600
700
800
900
1000
Detector 1-360nmOpuntia 2Jul2611018.dat
• Flavonoids HPLC-DAD-UV 360nm
Phytochemical composition
• Fatty acids
•palmitic acid • octadecadienoic acid
OPUNTIA - BASED NATURAL EXTRACTS
Both Opuntia extracts inhibited HT29 cell growth in a dose dependent manner.
• Antiproliferative effect
Dose response curves
Note: Incubation time- 24 hours
ED50 values ROS generation
Note: Extracts concentration- 0.5mg/mL
OR Extract OFI Extract OR Extract OFI Extract
Opuntia rubusta extract was the most effective in inhibiting HT29 cell growth – lowest ED50 value.
The antiproliferative effect of Opuntia extracts is probably related with the ROS generation at a cellular level
- Opuntia rubusta extract - Opuntia ficus indica extract
OPUNTIA - BASED NATURAL EXTRACTS
Opuntia extracts exhibited different responses on cell cycle arrest, which could be related with the distinct composition of samples:
• Opuntia robusta extract induced cell cycle arrest into G1
• Opuntia ficus indica extract induced cell cycle arrest in S phase
• Cell cycle arrest
Note: Incubation time- 24 hours; extracts concentration-ED50 value
OR Extract OFI Extract
Effect of betalains on cell cycle arrest
Effect of phytochemicals on cell cycle arrest
• Betanin– G0/G1 phase (myeloid leukemia cell line- K562)
(Sreekanth et al., 2007)
• Isorhamnetin– G2 and S phase (colon cell line, HCT-116) (Jaramillo et al., 2010)
•Quercetin–S phase (colon cell line, SW480) (Richter et al., 1999)
CORK - BASED NATURAL EXTRACTS natural extracts provided by Corticeira AMORIM, S.G.P.S., S.A (NutraCork project, QREN)
Cork extracts are rich phytochemicals
Phytochemical composition
CORK E1
CORK E2 Total Phenolics 116 mg GAE/g
• Cork E1- polyphenols and triterpenes
Triterpenes
Betulinic acid Ursolic acid
Friedelin Lupeol
• Cork E2 – polyphenols (phenolic acids and ellagitanins)
Minutes
10 20 30 40 50 60 70 80 90 100
mAU
0
50
100
150
200
250
300
350
400
450
500
mAU
0
50
100
150
200
250
300
350
400
450
500
Detector 1-280nmÁcido Elágico 45ppmNov 2612003.dat
Detector 1-280nmAmostra 6 Dil. 1:5Nov 2612004.dat
1- Gallic acid
2- Ellagic acid
- Ellagitanins
1
2
Ellagic acid
Minutes
0 10 20 30 40 50 60 70 80 90 100
mAU
0
5
10
15
20
25
30
35
40
45
50
55
60
65
70
75
80
mAU
0
5
10
15
20
25
30
35
40
45
50
55
60
65
70
75
80Detector 1-280nmNUC 183 (Conc.)Set2512010.dat
Total Phenolics 2.9 g GAE/L
Ellagic acid
CORK - BASED NATURAL EXTRACTS
Both cork extracts inhibited cancer cell growth in a dose dependent manner
ED50 = 3 mL extract/mL
• Antiproliferative effect
ED50 = 0.25 mg extract/mL
Note: Incubation time- 24 hours
CORK E1
CORK E2
CORK - BASED NATURAL EXTRACTS
Cork extracts exhibited different responses on cell cycle moduation, which could be related with the distinct composition of samples:
• Cork E1 extract induced cell cycle arrest into G1
• Cork E2 extract induced cell cycle arrest in S and G2/M phases
• Cell cycle arrest
Note: Incubation time- 24 hours; C Cork E1=2.4%; C Cork E2= 0.22mg/mL
Effect of phenolics on cell cycle arrest
Effect of triterpenes on cell cycle arrest
• Betulinic acid – G1 phase
• Ursolic acid- G1 phase
• Ellagic acid– S phase (HT29 cells)
• Gallic acid- S phase (HT29 cells)
• Ellagitanins- G0/G1 and G2/M phases (HT29 cells)
Kasimsetty et al.(2010)
Khan SA (2009)
Preliminary experiments
in HT29
This study demonstrates that cherry, cactus pear, olive and cork-based natural extracts inhibit the growth of HT29 through cell cycle modulation.
Natural extracts Induction of cell
cycle arrest Induction of cell
cycle arrest Compounds
CHERRIES POH-RICH EXTRACT
G1
OLIVE HT-RICH EXTRACT
OLIVE LT-OL-RICH EXTRACT
G1
S and G2/M
Perillyl alcohol (monoterpene)
G1
G1 Hydroxytyrosol (phenolic acid)
S Oleuropein (tyrosol esters)
G2/M Luteolin (flavonoid)
OPUNTIA RUBUSTA EXTRACT
OPUNTIA FICUS EXTRACT
Betanin (betaleins)
G1 G1 ?
S ? Quercetin (flavonoid)
G1 Betulinic acid and Ursolic acid (triterpenes)
Isorhamnetin (flavonoid)
S and G2/M ?
? .....
S
CORK EXTRACT 1
CORK EXTRACT 2
G1
S and G2/M Ellagic and gallic acids (phenolic acids)
S
G0/G1 and G2/M Ellagitannins
The natural extracts used in this study have the potential to improve the research and development of new chemotherapeutic agents for colon cancer.
This study demonstrates that cherry, cactus pear, olive and cork-based natural extracts inhibit the growth of HT29 through cell cycle modulation.
Evaluation of other natural extracts and ingredients
Evaluation of more anticancer effects (induction of apoptosis, 3D cell-based assays, …)
Joana Poejo, Inês Silva
Dr. Ana Matias
Group Leader: Dr. Catarina Duarte
Nutraceuticals and Controlled Delivery
Lab IBET/ITQB-UNL
Financial Support: • FEDEP/COMPETE -QREN project “NUTRACork” (ref. 21597/2011) • Fundação para a Ciência e Tecnologia (FCT) - PTDC/AGR-AAM/099645/2008 project - PEst-OE/EQB/LA0004/2011 grant - REDE/1518/REM/2005
Analytical Chemistry Lab ITQB/IBET
Dr. Rosário Bronze
Polymer Processing and Supercritical
Technology Lab FCT-UC
Dr. Herminio de Sousa
Dr. Mara Braga, Dr. Inês Seabra
CORTICEIRA AMORIM, S.G.P.S., S.A.
(Portugal)
Dr. Susana P. Silva, Patrícia Correia
iBET is a private not for profit research organization in the area of biotechnology and life sciences.
Oeiras, Portugal
The largest Biotechnology Research Organisation in Portugal
Brings together as partners and collaborators, public institutions and private companies
Main
Activities
Health – Pharma
Agro – Industry
Plants – Forestry
Environment
Mission
Foster the competitiveness of its customers
and partners
Create wealth out of
knowledge of Chemistry,
Biochemistry and Biology
Agro – Industry
Processing Chemical
characterization Biological
characterization Formulation
Development of alternative green technologies for the isolation of natural of bioactive compounds with high added-value and application in food, cosmetic and pharmaceutical industries
• Nutraceuticals and Controlled Delivery Lab • Membrane Processes Lab
Development and application of cell-based assays
• Nutraceuticals and Controlled Delivery Lab • Animal Cell Technology Lab
Identification and quantification of several classes of compounds
• Nutraceuticals and Controlled Delivery Lab • Analytical Chemistry Lab
Development of adequate and efficient systems to : -Increase Shelf life and stability of the bioactive -Increase solubility -- Increase bioavailaibity - ….
• Nutraceuticals and Controlled Delivery Lab
e-mail: [email protected]
http://www.itqb.unl.pt/labs/nutraceuticals-and-delivery
12TH INTERNATIONAL CONFERENCE FUNCTIONAL FOOD INGREDIENTS AND NUTRACEUTICALS IN CHRONIC DISEASE: SCIENCE AND PRACTICE NOVEMBER 29-DECEMBER2 DALLAS, TX, USA