Mass Spectral (MS) and
Retention Time Index (RI) Libraries of GC-MS Metabolite Profiles
Library overview:
T_MSRI_ID.txt (version 01.03.2004; version 02):
Annotated GC-TOF-MS
spectra
Q_MSRI_ID.txt (version 01.03.2004):
Annotated quadrupole GC-MS spectra
T_MSRI_NS.txt (version 01.03.2004 ):
Non-supervised collection
of GC-TOF-MS spectra
of
plant species
Q_LJA_NS.txt
(version 01.03.2004):
Non-supervised
collection of quadrupole GC-MS spectra
of
Lotus japonicus (Regel)
K. Larsen
Q_LYC_NS.txt
(version 01.03.2004):
Non-supervised
collection of quadrupole GC-MS spectra
of
Lycopersicon esculentum Mill. and related wild
species
Library description (T_MSRI_ID, Q_MSRI_ID):
T_MSRI_ID.xls
(version 01.03.2004)
Methods:
M[1] (EITTMS):
Sampling: shock freezing in
liquid nitrogen
Extraction: hot (70°C) methanol/
water/ chloroform (approx. 4:1:2; v/v/v)
Fractionation: polar metabolites
liquid partitioning into
methanol/water (approx. 1:1; v/v), and chloroform (chloroform phase is
discarded).
Derivatization: =N-O-CH3 (methoxyamine
hydrochloride/ pyridine reagent, 20 mg / ml)
-Si(CH3)3
(N-methyl-N-(trimethylsilyl)-trifluoroacetamide, MSTFA reagent)
RI system: n-dodecane (RI 1200), n-pentadecane (RI 1500), n-nonadecane
(RI 1900), n-docosane (RI 2200), n-octacosane (RI 2800), n-dotriacontane
(RI 3200), n-hexatriacontane (RI 3600)
GC: GC 6890 (Agilent
Technologies,
Injection: 1
µl splitless, 230°C, 2 min pulse at 110 psi
Column: Rtx-5Sil
MS, 30 m x 0.25 mm ID with 10 m integrated guard column, 0.25 µm film thickness
(Restek GmbH,
Temperature program: 2 min at 80 °C, 15 min ramp to 350 °C, 2 min at 350 °C
Carrier gas: Helium,
1 ml min-1, operated by
electronic pressure control
MS: Pegasus II TOF-MS system (Leco,
Ionization: electron impact
Scanning: 6 spectra s-1 (m/z = 70-600)
Deconvolution: AMDIS (Automated Mass Spectral Deconvolution
and Identification System, National Institute of Standards and Technology,
Settings: adjacent peak
subtraction (2), resolution (medium), sensitivity (high), shape requirements (high)
Remarks: Pure reference
substances are processed without extraction and fractionation.
Method variants: - Omission of fractionation for
the analysis of a mixed
polar and lipophilic fraction
-
Omission of methoxyamination
M[2] (EIQTMS):
Sampling: shock
freezing in liquid nitrogen
Extraction: hot (70°C) methanol/
water/ chloroform (approx. 4:1:2; v/v/v)
Fractionation: polar metabolites
liquid partitioning into
methanol/water (approx. 1:1; v/v), and chloroform (chloroform phase is
discarded).
Derivatization: =N-O-CH3 (methoxyamine
hydrochloride/ pyridine reagent, 20 mg / ml), -Si(CH3)3 (N-methyl-N-(trimethylsilyl)-trifluoroacetamide, MSTFA)
RI system: n-dodecane
(RI 1200), n-pentadecane (RI 1500), n-nonadecane (RI 1900), n-docosane
(RI 2200), n-octacosane (RI 2800), n-dotriacontane (RI 3200), n-hexatriacontane
(RI 3600)
GC: GC 8000 or GC
8000 Top (ThermoQuest,
Injection: 1 µl splitless, 230°C, 2 min
Column: Rtx-5Sil MS, 30 m x
0.25 mm ID with 10 m integrated guard column, 0.25 µm film thickness (Restek GmbH,
Temperature
program: 1 min at 70 °C, 6 min ramp
to 76 °C, 45 min ramp to 350°C, 1 min at 350 °C, 10 min at 330°C
Carrier gas: Helium 1 ml min-1
MS: MD 800 MS, Voyager MS or
Trace MS (ThermoQuest, Manchester, UK), transfer line 250°C, ion source 200°C
Ionization: electron impact
Scanning: 2 spectra s-1
(m/z = 40-600)
Deconvolution: AMDIS (Automated Mass Spectral
Deconvolution and Identification System, National
Institute of Standards and Technology,
Settings: adjacent
peak subtraction (2), resolution (low), sensitivity (very low –medium), shape
requirements (low)
Remarks: Pure
reference substances are processed without extraction and fractionation.
Method variants: - Omission of fractionation for
the analysis of a mixed
polar and lipophilic fraction
-
Omission of methoxyamination
Citations:
C[1] Wagner
C, Sefkow M, Kopka J (2003).
Construction and application of a mass spectral and retention time
index database generated from plant GC/EI-TOF-MS metabolite profiles.
Phytochemistry 62(6) 887-900
C[2] Colebatch G, Desbrosses G, Ott T, Krussel L, Kloska S, Kopka J, Udvardi
M (2004).
Global changes in transcription orchestrate metabolic differentiation
during symbiotic nitrogen fixation in Lotus japonicus.
(in preparation)
Sample Contributions:
S[1] Sefkow M,
Institute of Organic Chemistry and Structure Analysis, Karl-Liebknecht-Str. 24-25, D-14476
S[2] Wagner C, Kopka J,
Max Planck Institute of Molecular Plant Physiology, Department Prof.
Willmitzer, Am Muehlenberg 1, D-14476
S[3] Draeger B,
Institute of Pharmaceutical Biology, Hoher Weg 8, D-06120
S[4] Richter A,
Institute of Ecology and Conservation Biology, Althanstrasse
14, A-1090
S[5] Gormann R,
S[6] Allison G,
S[7] Hause B,
S[8] Desbrosses G*, Udvardi M,
Max Planck Institute of Molecular Plant Physiology, Am Muehlenberg 1, D-14476
* Université
Montpellier 2, CC 002, Place Eugène Bataillon, F-34095 Montpellier Cedex 05, France
S[9] Kehr J,
Max Planck Institute of Molecular Plant Physiology, Department Prof.
Willmitzer, Am Muehlenberg 1, D-14476
S[10] Kraemer U,
Max Planck Institute of Molecular Plant Physiology, Am Muehlenberg 1, D-14476
S[11] Peña-Cortés
H,
Centro de Biotecnologia, Universidad Tecnica Federico Santa Maria, Av. Espana
1680, Casilla 110-V,
S[12] Kaplan F, Guy CL,
S[13] Krueger S, Kopka
J,
Max Planck Institute of Molecular Plant Physiology, Department Prof.
Willmitzer, Am Muehlenberg 1, D-14476
S[14] Kempa S, Hoefgen
R,
Max Planck Institute of Molecular Plant Physiology, Department Prof.
Willmitzer, Am Muehlenberg 1, D-14476
S[15] Schauer
N, Roessner-Tunali U*, Fernie A,
Max Planck Institute of Molecular Plant Physiology, Department Prof.
Willmitzer, Am Muehlenberg 1, D-14476
*
S[16] Strelkov S, Schomburg D,
S[17] Wasternak C
Mass spectral
Contributions:
MST[1] Kopka J,
Max Planck Institute of Molecular Plant Physiology, Department Prof.
Willmitzer, Am Muehlenberg 1, D-14476
MST[2] Schauer
N,
Max Planck Institute of Molecular Plant Physiology, Department Prof.
Willmitzer, Am Muehlenberg 1, D-14476
T_MSRI_ID.txt (version 01.03.2004):
Collection of 855 (1394 version 02) identified or annotated mass
spectral tags (MSTs).
This collection contains 632 (796 version 02) non-redundant MSTs of which 229 (241 version 02) are identified. Mass spectra were manually generated from GC-TOF-MS
chromatograms of standard addition experiments or of biological samples. Each MST has an index number (MPIMP-ID) and a
substance name. Non-identified MSTs are characterized by mass spectral match and name of
best matching substance in square brackets.
Method: M[1]
Citation: C[1]
Q_MSRI_ID.txt (version
01.03.2004):
Collection of 1166 identified or annotated mass spectral tags (MSTs). This
collection contains 574 non-redundant MSTs of which 306
are identified. Mass spectra were
manually generated from quadrupole GC-MS
chromatograms of standard addition experiments or of biological samples. Each MST has an index number (MPIMP-ID) and a
substance name. Non-identified MSTs are characterized by mass spectral match and name of
best matching substance in square brackets.
Method: M[2]
Citation:
T_MSRI_NS.txt (version
01.03.2004):
Non-supervised collection of 7534 MSTs
obtained by automated deconvolution.
This collection includes all erroneous deconvolutions
and contaminations typically observed in non-sample controls. No signal to
noise threshold was applied.
Method: M[1]
Sample Contribution: S[2]
MST Contribution: MST[1]
Citation: C[1]
Sample Description:
|
Experiment |
Species |
Cultivar/Ecotype |
Organ |
Sample Fresh Weight (mg) |
MST number |
|
|
|
|
|
|
|
|
1135ec03 |
Non-sample control |
|
|
|
265 |
|
1135ec23 |
Non-sample control |
|
|
|
201 |
|
1135ec61 |
Non-sample control |
|
|
|
132 |
|
1135ec05 |
Arabidopsis
thaliana (L.) Heynh. |
C24 |
Leaf |
1 |
368 |
|
1135ec24 |
Arabidopsis
thaliana (L.) Heynh. |
C24 |
Leaf |
16 |
450 |
|
1135ec06 |
Arabidopsis
thaliana (L.) Heynh. |
C24 |
Root |
2 |
336 |
|
1135ec25 |
Arabidopsis
thaliana (L.) Heynh. |
C24 |
Root |
10 |
409 |
|
1135ec07 |
Nicotiana
tabacum L. |
SNN |
Leaf |
3 |
370 |
|
1135ec26 |
Nicotiana
tabacum L. |
SNN |
Leaf |
11 |
445 |
|
1135ec08 |
Nicotiana
tabacum L. |
SNN |
Root |
3 |
306 |
|
1135ec27 |
Nicotiana
tabacum L. |
SNN |
Root |
10 |
477 |
|
1135ec13 |
Solanum
tuberosum L. |
Désirée |
Flower |
3 |
333 |
|
1135ec32 |
Solanum
tuberosum L. |
Désirée |
Flower |
10 |
482 |
|
1135ec09 |
Solanum
tuberosum L. |
Désirée |
Leaf |
1 |
381 |
|
1135ec28 |
Solanum
tuberosum L. |
Désirée |
Leaf |
14 |
424 |
|
1135ec10 |
Solanum
tuberosum L. |
Désirée |
Root |
3 |
369 |
|
1135ec29 |
Solanum
tuberosum L. |
Désirée |
Root |
14 |
399 |
|
1135ec12 |
Solanum
tuberosum L. |
Désirée |
Stolon |
3 |
259 |
|
1135ec31 |
Solanum
tuberosum L. |
Désirée |
Stolon |
14 |
447 |
|
1135ec11 |
Solanum
tuberosum L. |
Désirée |
Tuber |
1 |
272 |
|
1135ec30 |
Solanum
tuberosum L. |
Désirée |
Tuber |
18 |
409 |
Experimental:
Plants were cultivated on soil in
growth chambers with a maximum of 120 µmol photons m-2 s-1
at leaf surface. Potato (Solanum tuberosum) and tobacco (Nicotiana tabacum) plants were grown in
3 l-pots with a 16 h-light/ 8 h-dark regime changing from 22 °C during the day
to 18 °C at night and with relative humidity preset to constant 70%. Arabidopsis thaliana plants were kept
in 0.125 l-pots with identical illumination but changing from 60% humidity and
20 °C during the day to 75% humidity and 18 °C at night. Samples of plant organs were harvested at 2-6
h in the light period from flowering plants.
Root samples were prepared free of soil but not rinsed with water.
Q_LJA_NS.txt (version 01.03.2004):
Non-supervised collection of 6857 MSTs
obtained by automated deconvolution.
This collection includes all erroneous deconvolutions,
and contaminations typically observed in non-sample controls. No signal to
noise threshold was applied.
Method: M[2]
Sample Contribution: S[8]
MST Contribution: MST[1]
Citation: C[2]
Sample Description:
|
Experiment |
Species |
Cultivar/Ecotype |
Organ |
Sample Fresh Weight (mg) |
MST number |
|
||||
|
|
|
|
|
|
|
|
||||
|
2236bg10 |
Lotus japonicus |
|
Root lateral |
25-50 |
389 |
|
||||
|
2236bg14 |
Lotus japonicus |
|
Root lateral |
25-50 |
318 |
|
||||
|
2236bg20 |
Lotus japonicus |
|
Root primary |
25-50 |
481 |
|
||||
|
2236bg24 |
Lotus japonicus |
|
Root primary |
25-50 |
511 |
|
||||
|
2233bn14 |
Lotus japonicus |
|
Nodule |
25-50 |
42* |
|
||||
|
2233bg08 |
Lotus japonicus |
|
Nodule |
25-50 |
623 |
|
||||
|
2233bg14 |
Lotus japonicus |
|
Nodule |
25-50 |
707 |
|
||||
|
2336bg54 |
Lotus japonicus |
|
Flower |
25-50 |
449 |
|
||||
|
2236bg50 |
Lotus japonicus |
|
Flower |
25-50 |
749 |
|
||||
|
2236bg30 |
Lotus japonicus |
|
Leaf developing |
25-50 |
703 |
|
||||
|
2236bg34 |
Lotus japonicus |
|
Leaf developing |
25-50 |
593 |
|
||||
|
2236bg40 |
Lotus japonicus |
|
Leaf mature |
25-50 |
770 |
|
||||
|
2236bg44 |
Lotus japonicus |
|
Leaf mature |
25-50 |
564 |
|
||||
|
* partial |
|
|
|
|
|
|||||
|
|
|
|
|
|
|
|||||
Experimental:
Lotus japonicus GIFU B-129 seeds were scarified in liquid nitrogen (3x10
sec), sterilized in a 2% bleach solution for 10 minutes, rinsed five times with
sterile distilled water, then germinated and grown in coarse quartz sand in a
controlled environment (16 h day, 60% relative humidity, and 21/17°C
day/night temperate regime). Pots were watered daily with 1/4 B&D medium. Plants were inoculated when 7 days old with Mesorhizobium loti strain R7A and provided with 1mM
KNO3 for the first 2-3 weeks of growth.
Plant organs were harvested at 12-weeks, collected directly into liquid
nitrogen, and stored at -80°C. At each harvest plants were carefully pulled
from the quartz sand and a complete set of 6 organ samples prepared, i.e.
nodules, lateral and primary root, mature and developing leaves, and
flowers. Leaves were separated according
to morphological criteria into a group of young expanding leaves from the apex
of the plant and a group of mature fully expanded leaves from the middle of the
plant shoot. Senescent leaves were
discarded. Whole flowers were prepared
including all floral organs, petals, sepals, carpels,
stamen, and pollen. Lateral roots
without visible nodule primordia were collected,
followed by pink nodules sampled in a representative range various sizes. The
harvest was completed by preparing the primary root, i.e. 2 cm of the main root
directly below the hypocotyl. Only samples without nodules and lateral
roots were collected.
Q_LYC_NS.txt (version 01.03.2004):
Non-supervised collection of 15386 MSTs
obtained by automated deconvolution.
This collection includes all erroneous deconvolutions,
and contaminations typically observed in non-sample controls. No signal to
noise threshold was applied.
Method: M[2]
Sample Contribution: S[15]
MST Contribution: MST[1], MST[2]
Citation:
Sample Description:
|
Experiment |
Species |
Cultivar/Ecotype |
Organ |
Sample Fresh Weight (mg) |
MST number |
|
|||||||
|
|
|
|
|
|
|
|
|||||||
|
04019a49 |
Lycopersicon esculentum |
M82 |
Root |
100 |
474 |
|
|||||||
|
04019a50 |
Lycopersicon esculentum |
M82 |
Root |
100 |
525 |
|
|||||||
|
2352AI05 |
Lycopersicon esculentum |
M82 |
Leaf |
100 |
484 |
|
|||||||
|
2352AI10 |
Lycopersicon esculentum |
M82 |
Leaf |
100 |
710 |
|
|||||||
|
3090AU02 |
Lycopersicon esculentum |
M82 |
Green fruit |
200-250 |
467 |
|
|||||||
|
3090AU10 |
Lycopersicon esculentum |
M82 |
Green fruit |
200-250 |
470 |
|
|||||||
|
3090AU05 |
Lycopersicon esculentum |
M82 |
Orange fruit |
200-250 |
458 |
|
|||||||
|
3090AU13 |
Lycopersicon esculentum |
M82 |
Orange fruit |
200-250 |
433 |
|
|||||||
|
3090AU09 |
Lycopersicon esculentum |
M82 |
Red fruit |
200-250 |
508 |
|
|||||||
|
3090AU17 |
Lycopersicon esculentum |
M82 |
Red fruit |
200-250 |
422 |
|
|||||||
|
03363a02 |
Lycopersicon pennellii |
|
Fruit 45DAF* |
200-250 |
349 |
|
|||||||
|
03363a03 |
Lycopersicon pennellii |
|
Fruit 45DAF |
200-250 |
451 |
|
|||||||
|
03363a10 |
Lycopersicon chmielewskii |
|
Fruit 45DAF |
200-250 |
475 |
|
|||||||
|
03363a11 |
Lycopersicon chmielewskii |
|
Fruit 45DAF |
200-250 |
431 |
|
|||||||
|
03363a08 |
Lycopersicon hirsutum |
|
Fruit 45DAF |
200-250 |
410 |
|
|||||||
|
03363a09 |
Lycopersicon hirsutum |
|
Fruit 45DAF |
200-250 |
392 |
|
|||||||
|
03363a06 |
Lycopersicon parviflorum |
|
Fruit 45DAF |
200-250 |
397 |
|
|||||||
|
03363a07 |
Lycopersicon parviflorum |
|
Fruit 45DAF |
200-250 |
379 |
|
|||||||
|
03363a04 |
Lycopersicon pimpinellifollium |
|
Fruit 45DAF |
200-250 |
384 |
|
|||||||
|
03363a05 |
Lycopersicon pimpinellifollium |
|
Fruit 45DAF |
200-250 |
382 |
|
|||||||
|
3268au03 |
Lycopersicon pennellii |
|
Leaf |
100 |
461 |
|
|||||||
|
3268au15 |
Lycopersicon pennellii |
|
Leaf |
100 |
578 |
|
|||||||
|
3268au31 |
Lycopersicon chmielewskii |
|
Leaf |
100 |
615 |
|
|||||||
|
3268au37 |
Lycopersicon chmielewskii |
|
Leaf |
100 |
688 |
|
|||||||
|
3268au06 |
Lycopersicon hirsutum |
|
Leaf |
100 |
657 |
|
|||||||
|
3268au18 |
Lycopersicon hirsutum |
|
Leaf |
100 |
731 |
||||||||
|
3268au16 |
Lycopersicon parviflorum |
|
Leaf |
100 |
689 |
||||||||
|
3268au28 |
Lycopersicon parviflorum |
|
Leaf |
100 |
710 |
||||||||
|
3268au05 |
Lycopersicon pimpinellifollium |
|
Leaf |
100 |
602 |
||||||||
|
3268au29 |
Lycopersicon pimpinellifollium |
|
Leaf |
100 |
689 |
||||||||
|
|
|
|
|
|
|
|
|||||||
*DAF (days after flowering)
Experimental:
Tomato plants of accession numbers LA1589 (L. pimpinellifolium), LA2133 (L. parviflorum),
LA1028 (L. chmielewskii), LA1777 (L. hirsutum) and LA0716 (L. pennellii)
were obtained from the true-breeding monogenic stocks maintained by the Tomato
Genetics Stock Centre (
Samples were taken 6 h into the light period from
mature fully developed leaves of 6-week-old plants. Fruit samples were taken
21DAF, 42DAF and at breaker stage exclusively from pericarp
tissue after rapid removal of the epidermis.
Root samples were taken 6h into the light period
from hydroponically grown tomato plants of accession
number LA2706 (Lycopersicon
esculentum cv. Moneymaker).
Plants were grown in tomato complete solution (Ca(NO3)2
1,25Mol m-3, KNO3 1,5 Mol m-3, MgSO4 0,75Mol
m-3, K2HPO4 0,83Mol m-3, FeEDTA 0,05Mol m-3, H3BO3 11,6µmol m-3,
MnSO4 2,4µmol m-3,
ZnSO4 0,2µmol
m-3, CuSO4 0,1µmol
m-3, NaMoO4 0,1µmol
m-3) under a 16h day/ 8h night regime with 250µmol photons m-2s-1
at 22°C/day and 20°C/night.