Information
-
Patent Grant
-
6573492
-
Patent Number
6,573,492
-
Date Filed
Tuesday, December 26, 200023 years ago
-
Date Issued
Tuesday, June 3, 200321 years ago
-
Inventors
-
Original Assignees
-
Examiners
- Lee; John R.
- Wells; Nikita
Agents
-
CPC
-
US Classifications
Field of Search
US
- 250 282
- 250 281
- 250 283
- 250 292
- 073 2322
-
International Classifications
-
Abstract
In a spectrometric analysis method and an apparatus implementing the method, a data base storing spectral data sets of respective standard substances, which are obtained by analyzing these standard substances in advance, each spectral data set including a name of a substance, its MS1 spectral data and MS2 spectral data, is constructed; and MS2 spectral data sets obtained by MS2 analysis of a sample are compared with MS2 analysis spectral data sets stored in the data base.
Description
BACKGROUND OF THE INVENTION
The present invention relates to a mass spectrometer including an ion trap, and a mass spectrometric analysis method performed in the mass spectrometer.
A mass spectrometer is an analytical instrument which charges sampled molecules of a measured object, and measures the mass number to electrical charge ratio of the generated ions, and an ion current, as mass spectral data. Since a substance possesses a specific molecular mass related to the kinds and number of atoms composing the substance, by obtaining the mass spectral data of the substance, it is possible to obtain important information to specify the substance. Further, since a mass spectrometer can be directly connected to a chromatography apparatus such as a gas or liquid chromatograph measurement device, a capillary electrophoresis chromatograph measurement device, and so forth, it can be used as a detector of high sensitivity, which is capable of obtaining various kinds of qualitative information, for a chromatography apparatus.
Recently, concern for environmental problems, health of a human body, etc. has grown, and a chromatograph direct-coupled type mass spectrometer has been used in various fields such as in checking for harmful organic compounds included in clean water, waste water, foods, etc., assessing the safety of a developed new drug, and so forth. Requirements for such an analytical instrument are as follows.
(1) It has a high sensitivity, and can perform a quantitative analysis with the analytical instrument.
(2) It is possible to obtain qualitative information enough to specify a substance certainly.
(3) It can remarkably reduce the work for a sample preparation, which is necessary in the measurement of a sample, to remove impurities which are not to be analyzed.
(4) Since a pesticide to be analyzed includes ten to sixty components, the analytical instrument is required simultaneously to analyze as many substances as possible by a single sample injection.
Specifically, in order to achieve the requirement (2), mass spectral data of standard substances are measured and stored in advance. On the other hand, a mass spectrum of the substance corresponding to each peak which has appeared in a chromatograph of a sample, is obtained, and a standard substance which has a mass spectrum coinciding with the measured mass spectrum corresponding to each in the chromatograph of the sample, is searched. Further, it is determined that if there are substances which have the mass spectra highly coinciding with the measured spectra of the peak substances in the chromatograph of the sample, respectively, the sample includes these substances.
In comparison to examine the coincidence between mass spectra of standard substances and those of respective peak substances in a sample, it frequently occurs that mass spectra of peak impurity substances included in the sample are measured, the impurity substances being not includes in the standard substances, and this causes deterioration of the measurement accuracy in the comparison results. If an atmospheric-pressure ionization method is used for ionizing a sample to be analyzed by a mass spectrometer, the obtained mass spectrum is generally a simple spectrum in which the peak corresponding to the molecular number of a sample has the highest intensity. Although the feature of the atmospheric-pressure ionization method is effective to confirm the molecular number of a sample, since there is generally a smaller number of peaks due to bond-cleavage ions in a mass spectrum obtained by using this ionization method in comparison with that obtained by using an electron impact ionization method, the mass spectrum obtained by using the atmospheric-pressure ionization method gives poor information to identify a sample, in the case where the identification of the sample is performed by comparing measured mass spectra of the sample with those of standard substances. Generally, the atmospheric-pressure ionization method is used for an ionization chamber connected to a liquid chromatograph, that is, an LC (Liquid Chromatograph)/MC (mass spectrograph) system, and the electron impact method is used for an ionization chamber connected to a gas chromatograph, that is, GC (Gas Chromatograph)/MC (mass spectrograph) system. Here, in the LC/MC system, after obtaining a mass spectrum for a definite range of mass only, it is very difficult to specify components of a sample.
To solve the above problem, what has been performed is, components of a sample are identified by specifying a representative mass number of each component of the sample and performing MS
n
analysis with regard to ions of the mass number, in order to increase spectral information on the sample.
In Japanese Patent Application Laid-Open Hei. 10-142196, it is disclosed that MS
1
analysis and MS
n
analysis are carried out in succession.
In the MS
n
analysis, ions of a specified mass number in ions, which have been introduced into a mass spectrograph, are selected. Then, energy is given to these selected ions by making them collide with neutral particles, and they are cleaved. Further, respective groups of the cleaved ions are sent to a detector in order of the mass number of the groups, and mass spectral data of each group of ions is obtained. Mass spectral data obtained by sending ions, which have been introduced into the mass spectrograph, to the detector without causing any reaction in these ions, is called simply MS spectral data, or MS
1
spectral data. On the other hand, mass spectral data of the above cleaved ions which have received the cleavage reaction of one stage, is called MS
n
spectral data. Moreover, by sending the selected ions to the detector after causing cleavage reactions in the selected ions, which have been introduced into the mass spectrograph, in multiple stages, data of MS
3
, MS
4
, or MS
5
, can be obtained. Since there is a portion in a molecule in which a cleavage easily occurs due to the structure of the molecule, even if the molecular number of a sample is equal to that of another sample, it is possible to distinguish samples of the same molecular number by comparing the respective spectral data of ions of the samples of different structures, which have received the cleavage reactions of multiple stages. Therefore, even if spectral information enough to specify a sample cannot be obtained by using usual MS data, the sample can be identified by using MS
n
data. Further, since the specific kind of ions are selected and cleaved, and MS
2
spectrum of the cleaved ions is obtained, the peaks existing in the spectral data, which are caused by impurities, can be excluded.
Although the above MS
n
analysis is excellent with regard to exclusion of influences due to impurities, and improvement of accuracy in substance-specification, it is necessary to specify the mass number of target ions to be cleaved, in advance, in order to perform the MS
n
analysis. If the analysis concerning a known substance is performed, it is easy to specify the mass number of target ions to be cleaved. However, if a sample whose components are unknown is analyzed, since the mass number of ions to be cleaved cannot be specified, it is necessary to perform the MS
n
analysis by determining the mass number of the ions to be analyzed, after obtaining total spectral information on the sample, by measuring MS
1
spectral data for a predetermined range of mass number once only.
In such an analysis, the task of the user is heavy, and the analysis takes much time. Particularly, in the LC/MC system using the atmospheric ionization method, since the MS
n
analysis is almost indispensable for the substance-specification, it is desirable that the MS
n
analysis be smoothly or efficiently performed.
Moreover, the kinds of ionized components of a sample, which have been introduced into a mass spectrograph from a chromatograph, change moment by moment. Therefore, the kind of ionized component which is analyzed by the MS
n
analysis has already changed from that of the ionized component which should have been analyzed by the MS
n
analysis, in measurement processing in which the MS
n
analysis is performed after MS
n
spectral data for a predetermined range of mass number once only, which in turn causes erroneous results of the analysis. That is, it occurs that the analysis performed by the mass spectrograph cannot follow changes in the kinds of ionized components in the sample.
SUMMARY OF THE INVENTION
The present invention has been achieved in consideration of the above-described problems, and is aimed at providing a mass spectrometric analysis method, and an apparatus implementing the method, which is capable of accurately specifying substances included in a sample by using mass spectral data obtained by MS
2
analysis.
To achieve the above objective, the present invention provides a spectrometric analysis method and an apparatus implementing the method, in that a data base storing spectral data sets of respective standard substances, which are obtained by analyzing these standard substances in advance, each spectral data set including a name of a substance, its MS
1
spectral data and MS
2
spectral data, is constructed; and MS
2
spectral data sets obtained by MS
2
analysis of a sample are compared with MS
2
analysis spectral data sets stored in the data base.
BRIEF DESCRIPTION OF THE DRAWINGS
FIG. 1
is a schematic diagram of the composition of a mass spectrometric analysis apparatus of an embodiment according to the present invention.
FIG. 2
is a flowchart of amass spectrometric analysis method of embodiment 1 according to the present invention.
FIG. 3
is a flow chart of a mass spectrometric analysis method of embodiment 2 according to the present invention.
FIG. 4
is an example of contents of a data base.
FIG. 5A
is an example of a condition-setting picture used in embodiment 1.
FIG. 5B
is an example of a condition-setting picture used in embodiment 2.
FIGS. 6A
,
6
B, and
6
C are figures conceptually illustrating the analysis processing performed in embodiment 1.
FIG. 7
is an example of a picture displaying results of the analysis performed in embodiment 1.
FIGS. 8A and 8B
are figures conceptually illustrating the analysis processing performed in embodiment 2.
FIG. 9
is an example of a picture displaying results of the analysis performed in embodiment 2.
DETAILED DESCRIPTION OF THE EMBODIMENTS
Hereafter, the embodiments according to the present invention will be explained in detail with reference to the drawings.
In
FIG. 1
, the composition of a mass spectrometric analysis apparatus which is used in the embodiments according to the present invention is shown, and in
FIG. 2
, the detailed composition of the data processing unit is shown.
As shown in
FIG. 1
, the mass spectrometric analysis apparatus used in this embodiment, includes a chromatography unit
10
for separating components contained in a sample, an ionization chamber
14
for ionizing each separated component of the sample, a mass spectrometric analysis unit
15
for performing mass spectral analysis of ions which have been introduced from the ionization chamber
14
, a detection device
16
for detecting ions which have passed through the analysis unit
15
. The chromatography unit
10
includes a sample-introducing device
11
into which a sample is injected, an analysis column
13
for separating components contained in the sample, and a solvent-feed unit and a pump which are used (not shown in this figure) for feeding solvent which transfers the components of the sample. The sample-introducing device
11
and the analysis column
13
, and the analysis column
13
and the ionization chamber
14
, are connected to each other by respective pipes
12
.
Further, the mass spectrometric analysis unit
15
of this embodiment includes a control unit
17
and a data processing unit
19
. Signal wires
18
connect the mass spectrometric analysis unit
15
to the ionization chamber
14
and the control unit
17
, the detection device
16
for detecting the density of ions of each mass number, to the data processing unit
19
, and the control unit
17
to the data processing unit
19
.
The data processing unit
19
receives mass spectral data detected by the detection device
16
via the signal wire
18
, processes the received data, and display the results of the processing on a display screen
20
. Further, the data processing unit
19
sends control signals of predetermined procedures to the control unit via the signal wire
18
. Furthermore, the data processing unit
19
includes an input device (not shown in this figure) such as a keyboard used for an operator to input various setting information, and a pointing device (not shown in this figure) for moving a cursor on the display screen
20
in an image display device.
The control unit
17
controls the voltage applied to the mass spectrometric analysis unit
15
and so forth, in response to the control signals sent from the data processing unit
19
.
The mass spectrometric analysis unit
15
of this embodiment uses an ion trap composed of a ring electrode and a pair of end cap electrodes. Further, the mass spectrometric analysis unit
15
generates a three-dimensional quadrupole electric field in a space surrounded by the ring electrode and the pair of end cap electrodes by applying high-frequency voltage to the ring electrode. The components of the sample, which have been ionized in the ionization chamber
14
, are introduced into the above space in the spectrometric analysis unit
15
, and are held in the generated three-dimensional quadrupole electric field once. Then, when MS
1
spectral data are obtained, ions are ejected to the detection device
16
in the order of increasing mass number by scanning the applied high-frequency voltage, and they are detected. The detected ion-density signal is sent to the data processing unit
19
, and is recorded as a total ion chromatogram (TIC) which represents the change in time of the ion signal strength. Also, a mass spectral data of changes in the ion signal strength with respect to each mass to charge ratio (m/Z) is obtained and stored at each time step.
Further, when MS
n
spectral data are obtained, first, ions of a specified mass number are held in the ion trap in the mass spectrometric analysis unit
15
, and ions of the other mass numbers are removed. This state can be easily implemented by applying high-frequency voltage, such as to cause the resonance state of the ions to be removed, to these ions. Next, CID (Collision Induced Dissociation) reactions are caused in the ions held in the ion trap by adding energy to these ions, which is implemented by applying the voltage of frequency equal to (or different from) the resonant frequency of motion of the ions. The ions cleaved by the CID reactions are ejected to the detection device
16
and detected. Thus, the MS
n
spectral data can also be obtained.
The mass spectrometric analysis for obtaining MS
1
spectral data and MS
n
spectral data spectral data can be performed by (1 s-3 s)/time. On the other hand, since the introduction of a sample from the chromatography unit
10
into the mass spectrometric analysis unit
15
is continued for about 10 minutes, this sample-introduction time is remarkably longer than the analysis time. Also, the sample introduced from the chromatography unit
10
into the mass spectrometric analysis unit
15
is separated into the respective components. Therefore, even if MS
1
spectral data and MS
n
spectral data are obtained in succession, as mentioned above, since the analysis time is sufficiently shorter than the sample-introduction time, the MS
1
spectral data and MS
n
spectral data of one component of the sample can be obtained within the introduction time of one component.
The present invention makes use of the feature of an ion trap, in which ions can be cleaved by controlling the electric field in the ion trap.
In the following, the embodiment 1 will be explained with reference to the drawings.
Embodiment 1:
This embodiment is an analysis which is effective for specifying components of a unknown sample.
FIG. 2
shows a flow chart of the processing performed in this embodiment.
First, in step S
1
, a measurement condition-setting picture such as that shown in
FIG. 5A
is displayed on the display screen
20
, and a user inputs each measurement condition. The main measurement conditions are “RANGE OF MASS NUMBER TO BE ANALYZED” and “HEIGHT-ORDER NUMBER OF PEAK TO BE ANALYZED”. The conditions of “PEAK TO BE EXCLUDED” and “THRESHOLD VALUE TO SIGNAL STRENGTH” are prepared to improve mass analysis, and it is possible that these conditions are not always set. Meanwhile, although mass number should be correctly described as mass to charge ratio (m/Z), this ratio m/Z is described as mass number in this specification for simplicity.
A range of mass number of ions whose MS
2
spectral data are obtained is set to “RANGE OF MASS NUMBER TO BE ANALYZED”. In this case, the range of mass number “200-400” is set. Further, it is set to “HEIGHT-ORDER NUMBER OF PEAK TO BE ANALYZED” what peaks in the peaks of the MS
1
spectrum measured in the range of 200-400 which is set in “RANGE OF MASS NUMBER TO BE ANALYZED”, is analyzed for MS
2
analysis. In this case, #1 is input to this condition, and this means that ions corresponding to the highest peak in the measured MS
1
spectrum are analyzed for MS
2
analysis. In “PEAK TO BE EXCLUDED”, a peak which should not be analyzed for MS
2
analysis is designated. In this case, since the value of 250 (m/Z) is input, even if a peak of this mass number is detected in the measured MS
1
spectrum, ions corresponding to this peak are not analyzed for MS
2
analysis. Sometimes, a substance such as Teflon which is used for the pipe
12
, is mixed in a sample, and is detected as an impurity substance. The providing of the condition “PEAK TO BE EXCLUDED” is effective for preventing detection of such an impurity substance. The condition “THRESHOLD VALUE TO SIGNAL STRENGTH” is provided to designate the minimum signal strength of candidate peaks to be analyzed for MS
2
analysis. By providing this condition, peaks of noise level can be excluded from object peaks to be analyzed for MS
2
analysis.
Next, the analysis of the sample starts. The sample injected from the sample-introducing device
11
is separated into each component substance (referred to simply as component or substance) by the analysis column
13
, and each separated component is sent to the ionization chamber
14
. Further, the mass spectrometry of the component ionized in the ionization chamber
14
is performed by the mass spectrometric analysis unit
15
, and the ionized component is detected by the detection device
16
. In this embodiment, in step S
2
, while MS
1
analysis and MS
2
analysis are alternately performed, the mass spectrometry is continued until the introduction of the sample from the chromatography unit
10
is completed. Here, the analysis is performed for only a group of ions, which satisfies the analysis conditions set in step S
1
.
FIGS. 6A
,
6
B, and
6
C conceptually illustrate the processing executed in step
2
. Also,
FIG. 6A
shows a total ion chromatograph (TIC) obtained in the MS
1
analysis. The MS
1
analysis is performed at each measurement point by a predetermined period (
3
s
in this example). As shown in FIG.
6
B and
FIG. 6C
, the MS
2
analysis of the designated peak in the MS
1
spectrum obtained at each measurement point is performed within each period between two measurement points.
All the obtained MS
1
and MS
2
spectral data are stored in a memory situated in the data processing unit
19
.
Next, in step S
3
, spectral data sets of substances, which satisfy the analysis conditions set in step S
1
, are selected by searching MS
1
spectral data sets in a data base stored in the data processing unit
19
.
Here, the above data base is conceptually illustrated in FIG.
4
. In this data base, spectral data sets of respective standard substances, which are obtained by analyzing these standard substances, are stored in advance. Further, each spectral data set includes a substance name, its MS
1
spectral data, and MS
2
spectral data obtained by performing analysis for ions corresponding to characteristic peaks in the MS
1
spectrum. For example, the spectral data set of substance A in
FIG. 4
includes MS
1
spectrum having peaks {circle around (
1
)} and {circle around (
2
)} at 200 m/Z and 650 m/Z, and two MS
2
spectra obtained by performing analysis for ions corresponding to the peaks {circle around (
1
)} and {circle around (
2
)}.
The processing executed in step
3
is explained below for the case wherein the analysis conditions is shown in FIG.
5
A. Since object peaks are the highest peak in the MS
1
spectrum of each substance whose mass number is within the range of 200-400 m/Z (however, the peak at 250 m/Z is excluded), peak {circle around (
2
)} in the spectrum of substance A, peak {circle around (
1
)} in the spectrum of substance B, and peak {circle around (
3
)} in the spectrum of substance C, are selected as the object peaks.
Next, in step S
4
, each MS
2
spectrum obtained by the MS
2
analysis performed in step S
2
is compared with the respective MS
2
spectral data selected from the data base. That is, each MS
2
measured spectrum is compared with the respective MS
2
spectra corresponding to peak {circle around (
2
)} in the spectrum of substance A, peak {circle around (
1
)} in the spectrum of substance B, and peak {circle around (
3
)} in the spectrum of substance C, in turn. Since there are a plurality of components in the sample, plural types of MS
1
spectra are obtained over the whole retention time of the TIC output from the chromatography unit
10
. Each type of MS
1
spectrum basically corresponds to a component of a peak in the TIC. Therefore, each of the MS
2
spectra with regard to the measured plural types of MS
1
spectra is compared with the respective MS
2
spectra selected from the data base.
Last, in step S
5
, the name of the substance whose MS
2
spectrum most agrees with the MS
2
spectrum obtained in each time region (spanning each peak in the TIC), is displayed on the display screen
20
as the component of the sample, which corresponds to the time region in the TIC.
FIG. 7
shows an example of the above display.
According to this embodiment, components of a sample can be promptly specified by using MS
2
spectral data. Therefore, even if no more than very simple mass spectrum, which is obtained by MS
1
analysis such as that performed in a LC/MC system using the atmospheric ionization method, can be obtained, components of a sample can still be promptly and accurately specified.
Further, by designating the range of mass number of peaks in MS
1
spectrum, to be analyzed for MS
2
analysis, candidates of substances to be analyzed, which are stored in a data base, can be narrowed down.
In the following, the embodiment 2 will be explained with reference to the drawings.
Embodiment 2
This embodiment is effective for the case wherein the name of a component to be analyzed, in a sample, is designated in advance.
FIG. 3
shows a flow chart of the processing performed in this embodiment.
First, in step S
11
, a measurement condition-setting picture such as that shown in
FIG. 5B
is displayed on the display screen
20
, and a user inputs each measurement condition. The main measurement conditions to be input in this example are “NAME OF SUBSTANCE” and “IMPORTANT PEAK”. Further, in this example also, the condition “THRESHOLD VALUE TO SIGNAL STRENGTH” is prepared to improve mass analysis, and it is possible that this condition is not always set.
To “NAME OF SUBSTANCE”, the name of a substance whose presence in a sample is to be confirmed, is set. In this case, the name of substance B is set. Also, the mass number (m/Z) of the characteristic peak, which must appear in the mass spectrum of the substance B, is set to “IMPORTANT PEAK”. In this case, the value of 400 (m/Z) is set. Further, the value of 20% is set to “THRESHOLD VALUE TO SIGNAL STRENGTH”.
When the input data are set to “NAME OF SUBSTANCE” and “IMPORTANT PEAK”, spectral information on the set substance is displayed in the region under the region for “THRESHOLD VALUE TO SIGNAL STRENGTH” on the display screen
20
as shown in FIG.
5
B. In this case, since the name of substance B and the mass number 400 of the important peak are set, MS
1
spectral data and MS
2
spectral data with regard to the important peak are displayed. After the condition-input to the picture on the display screen
20
is completed, the user moves the cursor to the button “STORE”, and clicks it. Then the condition-setting is complete.
Next, the analysis of the sample starts. In this embodiment also, in step S
12
, while MS
1
analysis and MS
2
analysis are alternately performed, the mass spectrometry is continued until the introduction of the sample from the chromatography unit
10
is completed. Here, the MS
2
analysis is performed for ions corresponding to the important peak set in step S
11
. In this case, the MS
2
analysis is performed for the peak of 400 m/Z which is set in the picture shown in FIG.
5
B.
All the obtained MS
1
and MS
2
spectral data are stored in a memory situated in the data processing unit
19
.
Further, in step S
13
, amass chromatogram corresponding to the important peak set in step S
11
is obtained. In this case, this mass chromatogram corresponds to the TIC used for the MS
2
analysis of the peak at 400 m/Z. Also, a mass chromatogram obtained by extracting only the chromatogram component corresponding to the mass number 400 m/Z, in the MS
1
analysis of the sample, can also be used as the above mass chromatogram corresponding to the important peak to be obtained in step
13
.
Furthermore, in step
14
, the MS
2
spectrum obtained by the MS
2
analysis of each peak in the mass chromatogram corresponding to the important peak is compared with the spectrum of the substance set in step S
11
, which has been selected from the data base, shown in FIG.
4
.
Here, examples of; the mass chromatogram corresponding to the important peak, and the MS
2
spectra obtained by the MS
2
analysis of the respective peaks; are shown in FIG.
8
A and
FIG. 8B
, respectively. In
FIG. 8A
, the mass chromatogram corresponding to the peak of 400 m/Z is shown. This figure also indicates that three peaks a, b, and c, whose heights are greater than the set threshold value of signal strength of 20%, are discriminated. In FIG
8
B, the MS
2
spectra obtained by the MS
2
analysis of the peaks a, b, and c, are shown, respectively. In step
14
, each of the MS
2
spectra shown in
FIG. 8B
is compared with the MS
2
spectrum {circle around (
1
)} of substance B selected from the data base shown in FIG.
4
.
Lastly, in step
15
, the retention time of the peak in the mass chromatogram, whose spectrum most agrees with the spectrum of substance B in the data base, is specified, and the MS
1
spectrum and MS
2
spectrum of the component at the specified retention time are shown on the display screen
20
. Thus, the whole processing ends.
An example of the displayed picture of the results is shown in FIG.
9
. As shown in
FIG. 9
, items displayed in this picture are “NAME OF SUBSTANCE” and “IMPORTANT PEAK” set in step S
11
, the TIC for all mass number, the mass chromatogram of the set important peak, and the MS
1
spectrum and MS
2
spectrum of the component at the specified retention time. The arrows shown in the TIC for all mass number, the mass chromatogram of the set important peak indicate the specified retention time.
In this embodiment, since an object substance to be analyzed is predetermined, by performing MS
2
analysis for only an important peak, which is designated in peaks in the MS
1
spectrum of a sample, and comparing each of the M
2
spectra obtained by the analysis with the MS
2
spectrum of the object substance, it is possible to confirm the retention time of the object substance included in the sample quickly and accurately.
In the above two embodiments, spectral data obtained by MS
1
and MS
2
analyses are used to specify components in a sample. However, spectral data obtained by MS
n
analysis (n=3, 4, . . . ) can also be used. As n increases, although the amount of spectral data stored in the data base greatly increases, which in turn will increase the memory size in the data processing unit
19
, and cause deterioration of processing speed of the unit
19
, the accuracy of analysis can be improved.
As described above, one main feature of the present invention is that a set of MS
2
spectra according to respective key peaks in MS
1
spectrum of each standard substance is prepared in a data base. By preparing such a data base and performing the analysis methods described in the above embodiments, even a mass analysis apparatus, such as an LC/MC system using the atmospheric ionization method, in which spectral information obtained from mass spectral data measured by MS
1
analysis is poor, can specify components in a sample promptly and accurately. Thus, the accuracy of specifying components in a sample can be increased. Also, in the case wherein it is confirmed that a specified substance is included in a sample, the presence of this substance in the sample can be efficiently determined.
Moreover, in accordance with the present invention, since MS
2
spectral data can be accumulated in a single MS
1
analysis, the sample analysis can easily follow changes in components of a sample, which has been introduced from a chromatograph, and a real-time analysis has become possible. Further, since it is not necessary to perform re-analysis for MS
2
analysis, the analysis according to the present invention is very effective for analyzing a valuable sample.
Claims
- 1. A mass spectrometric analysis method having a standard data base storing MS1 mass spectrometric data for an MS1 analysis and MS2 mass spectrometric data for an MS2 analysis and performing said MS1 analysis and MS2 analysis by using an ion trap capable of trapping ionized components of a sample, which have been introduced into a mass spectrometric analysis unit, said method comprising the steps of:setting analysis conditions for performing said MS2 analysis; obtaining mass spectra for said MS1 analysis and said MS2 analysis while alternately performing said MS1 analysis and MS2 analysis for said ionized components which satisfy said analysis condition set; selecting said MS1 mass spectrometric data and said MS2 mass spectrometric data satisfying said set analysis conditions from said standard data base; and comparing said mass spectrum obtained by said MS2 analysis with said selected MS2 mass spectrometric data for MS2 analysis from said standard data base.
- 2. A mass spectrometric analysis method according to claim 1, wherein a range of mass number to charge ratio, in which MS2 analysis is performed, and the position of at least one characteristic peak in respective spectral data sets to be obtained, at which ionized components of said sample are analyzed for MS2 analysis, are set to said analysis conditions.
- 3. A mass spectrometric analysis method according to claim 1, wherein the position of an excluded peak in respective spectral data sets at which ionized components of said sample are not analyzed for MS2 analysis, and a threshold value of signal strength, only ions of signal strength higher than said threshold value being analyzed for MS2 analysis, are set to said analysis conditions.
- 4. Amass spectrometric analysis method according to claim 1, wherein said comparison is performed for all the obtained spectral data sets, and the substance whose spectrum most agrees with one of said obtained spectral data sets is output as a result of said comparison.
- 5. A mass spectrometric analysis method having a standard data base storing MS1 mass spectrometric data for MS1 analysis and MS2 mass spectrometric data for MS2 analysis and performing said MS1 analysis and MS2 analysis by using an ion trap capable of trapping ionized components of a sample, which has been introduced into a mass spectrometric analysis unit, said method comprising the steps of:setting a mass number to charge ratio (m/z); obtaining mass spectra for said mass number to charge ratio while alternately performing said MS1 analysis and MS2 analysis; and judging a peak of said mass spectrum of said set mass number to charge ratio (m/z) and comparing said mass spectrum at said peak obtained by said MS2 analysis with said selected MS2 mass spectrometric data for MS2 analysis from said standard data base corresponding to said ionized component being said peak of said set mass number to charge ratio (m/z).
- 6. A mass spectrometric analysis method according to claim 5, wherein a name of a substance is et along with said mass to charge ratio, and respective said mass spectrum sets corresponding to said selected peaks in said mass chromatogram are compared with a MS2 mass spectrometric data set of said set name of said substance in said data base.
- 7. A mass spectrometric analysis method according to claim 6, wherein a retention time at which ions of a component in said sample, equal to said set substance, are detected in said chromatogram, is displayed as a result of said comparison.
- 8. A mass spectrometric analysis apparatus including an ion chamber for ionizing components of a sample, which have been introduced, a mass spectrometric analysis unit for trapping and cleaving said ionized component, and performing mass spectrometric analysis of said ionized component, a detection device for detecting ionized components which have been ejected from said mass spectrometric analysis unit, a data processing unit for processing information sent from said detection device, an input device for inputting analysis conditions set by a user, and a display device for display results of said data processing, said apparatus comprising:a standard data base storing MS1 mass spectrometric data for MS1 analysis and MS2 mass spectrometric data for MS2 analysis corresponding to ionized components; wherein said display device displays said analysis conditions for said MS2 analysis inputted from said input device mass spectrum sets of said introduced components of said sample are obtained while alternately performing MS1 analysis and MS2 analysis, and MS2 spectral data sets obtained by said MS2 analysis based on said condition inputted from said input device are compared with MS2 analysis spectrometric data sets in said data base.
- 9. A mass spectrometric analysis apparatus according to claim 8, wherein a picture for setting a range of mass number to charge ratio, in which MS2 analysis is performed, and the position of at least one characteristic peak in spectral data, at which ionized components of said sample are analyzed for MS2 analysis, is displayed on said display device.
- 10. A mass spectrometric analysis apparatus according to claim 9, wherein said data processing analysis creates a mass chromatogram of ions at said peak at said ratio (m/Z) by using said results of mass spectrometric analysis for said sample, and displays said created mass chromatogram.
- 11. A mass spectrometric analysis apparatus according to claim 9, wherein regions for setting the position of an excluded peak in spectral data at which ionized components of said sample are not analyzed for MS2 analysis, and a threshold value of signal strength, only ions of signal strength higher than said threshold value being analyzed MS2 analysis, are displayed in said picture.
- 12. A mass spectrometric analysis apparatus according to claim 8, wherein a picture for setting a name of a substance to be analyzed, and a mass number to charge ratio (m/Z), a peak at said ratio being an important peak of analysis, is displayed on said display device.
Priority Claims (1)
Number |
Date |
Country |
Kind |
11-371361 |
Dec 1999 |
JP |
|
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Oct 1982 |
A |
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Whitehouse et al. |
Jan 2000 |
A |
6147344 |
Annis et al. |
Nov 2000 |
A |
Foreign Referenced Citations (1)
Number |
Date |
Country |
10-142196 |
May 1998 |
JP |