Mass spectrometry interface, a mass spectrometer and a mass spectrometry

Description

BACKGROUND OF THE INVENTION

1) Field of the Invention

This invention relates to a mass spectrometry interface, a mass spectrometer and a mass spectrometry, more particularly to a mass spectrometry interface, a mass spectrometer and a mass spectrometry preferably usable for a mass spectrometry of a liquid sample, a liquid chromatograph, or a biological sample and an ionization spectroscopic analysis

2) Description of the Prior Art

Conventionally, a Matrix-Assisted Laser Deposition Ionization (MALDI) method or an electro spray method is employed for measuring a mass spectrum of a nonvolatile large mass molecule, and thus, the mass spectrum measuring technique is being widely applied for chemical fields or biological fields.

In the MALDI method, for enhancing the ionization of a dissolved substance to be analyzed in its mass, a large amount of matrix reagent is added into the sample solution incorporating the dissolved substance, and then, the thus obtained liquid sample is dropped onto a given plate to be evaporated and crystallized. Then, the plate is introduced into a mass spectrometer and irradiated by a laser beam to ionize the dissolved substance for its mass spectrometry.

In the electro spray method, a high voltage is applied to a nozzle to emit the liquid sample incorporating the dissolved substance, and thereby, the solvent of the liquid sample is desorbed and the dissolved substance is ionized. Then, the ionized dissolved substance is directly introduced into a mass spectrometer to be analyzed in its mass.

In the above electro splay method, an electrolyte is added to the liquid sample in order to enhance the ionization of the dissolved substance. Moreover, methanol, acetinitrile or the like to destroy the structure of a water is incorporated in the liquid sample for enhancing the desorption.

However, in the MALDI method, the liquid sample incorporating the dissolved substance may be often denaturalized due to much matrix reagent. Therefore, the MALDI method can not be applied for a liquid sample chemically changeable in short time and a long time-continuous measurement such as a mass spectrometry of a liquid chromatograph.

The electro spray method can not be also applied for the chemically changeable liquid sample and the long time-continuous measurement due to the denature of the liquid sample through the high voltage application. Moreover, if it is attempted that the denature of the liquid sample is prevented, the kind of the usable solvent is restricted. And then, if an associative solvent is employed in order to prevent the denature of the liquid sample, the clusters generated from the solvent molecules adheres to the solute species, and thus, the noises due to the clusters are superimposed on the mass spectrometry results of the dissolved substance.

SUMMERY OF THE INVENTION

It is an object of the present invention to provide a new mass spectrometer and mass spectrometry without the above matters.

For achieving the above object, the first invention relates to a mass spectrometry interface to constitute a mass spectrometer which comprises a vacuum chamber with a laser beam inlet, a metallic rotation-translation drum installed in the vacuum chamber, a sample supplying nozzle to emit and stabilize a liquid sample incorporating a dissolved substance to be analyzed in its mass for and onto the rotation-translation drum, and a laser source to irradiate a laser beam onto the dissolved substance from the laser beam inlet and to ionize the dissolved substance.

The second invention relates to a mass spectrometer to directly achieve the above object which comprises the above mass spectrometry interface or the following preferred mass spectrometry interface, an ion accelerating electrode part, and an mass spectrometry part.

Moreover, the third invention relates to a mass spectrometry using the above mass spectrometry interface or the mass spectrometer, comprising the steps of:

evacuating up to a given vacuum degree the interior of a vacuum chamber of a mass spectrometry interface constituting a mass spectrometer,

emitting a liquid sample incorporating a dissolved substance to be analyzed in its mass for a rotation-translation drum from a sample supplying nozzle of the mass spectrometry interface and thereby, stabilizing the dissolved substance on the rotation-translation drum, and

irradiating a laser beam for the stabilized dissolved substance from a laser source of the mass spectrometry interface via a laser beam inlet formed at the vacuum chamber and thereby, ionizing the dissolved substance.

According to the first through third inventions, only the dissolved substance to be analyzed in its mass is isolated on the metallic rotation-translation drum installed in the vacuum chamber, and a laser beam is directly irradiated on the deposited substance. Therefore, the substance isolated on the metal surface is ionized at high efficiency, and thus, an extreme high sensitive and efficient mass spectrometry can be performed.

The dissolved substance can fixed continuously as a long spiral belt on the rotation-translation drum. Therefore, the mass spectrometer and mass spectrometry of the present invention can be preferably employed for a long time-continuous measurement such as a mass spectrometry of a liquid chromatograph.

Therefore, much matrix reagent is not required, different from the MALDI method, and a high voltage is not also required, different from the electro-spray method. As a result, the denature of the liquid sample can be prevented, and the noises due to the clusters can be also prevented.

BRIEF DESCRIPTION OF THE DRAWINGS

For better understanding of the present invention, reference is made to the attached drawings, wherein

FIGURE is a schematic view showing an embodiment of the mass spectrometry of the present invention.

DESCRIPTION OF THE PREFERRED EMBODIMENTS

FIGURE is a structural view schematically showing an embodiment of the mass spectrometry of the present invention.

The depicted mass spectrometry has a mass spectrometry interface

1

, an ion accelerating electrode part

2

and a mass spectrometry part

3

, according to the present invention.

The mass spectrometry part

1

, according to the present invention, has a vacuum chamber

10

with a laser beam inlet

14

, a rotation-translation drum

11

provided in the vacuum chamber

10

, a sample supplying nozzle

12

to emit a liquid sample incorporating a dissolved substance to be analyzed in its mass for the rotation-translation drum

11

, and a laser source

13

to ionize the dissolved substance deposited on the rotation-translation drum

11

.

Moreover, a nozzle

15

to enhance the ionization of the dissolved substance through the formation of an optical absorption layer made of an optical absorption material on the rotation-translation drum is provided. The nozzle

15

is not essential in the present invention, but it can develop the detection sensitivity of the mass spectrometry of the present invention.

The rotation-translation drum

11

has a double structure of a shaft

11

A and a thin titanium tube

11

B supported by spokes. A driving unit

17

to rotate and translate the rotation-translation drum

11

is provided on the outer surface of the upper chamber wall of the vacuum chamber

10

, and transmits its rotation and translation driving force to the drum

11

through the shaft

11

A.

The rotation-translation drum

11

may have another construction, but the above double structure is simple, so the drum

11

can be made to be light in its weight and the rotation and translation movement can be easily operated.

A cryopump

16

is positioned at the area denoted by a broken line in the vacuum chamber

10

, and thus, the solvent such as a water of the liquid sample is evacuated efficiently and the interior of the vacuum chamber

10

can be maintained at a relatively high vacuum degree.

Moreover, since a heating cap

18

is provided at the forefront of the sample supplying nozzle

12

, the condensation of the liquid sample due to the rapid temperature drop through its adiabatic expansion can be prevented when the liquid sample is emitted for the rotation-translation drum

11

in the vacuum chamber

10

. In a preferred embodiment, the liquid sample is maintained constantly at a temperature of not lower than 27° C. (300K).

Furthermore, since a filter

12

A is provided in the sample supplying nozzle

12

, only the dissolved substance particles having a given size or smaller are passed through the nozzle

12

and emitted for the rotation-translation drum

11

. Thereby, the stuffiness of the sample supplying nozzle

12

is prevented, and the dissolved substance is fixed onto the metal surface of the rotation-translation drum

11

idealistically. As a result, the ionization efficiency can be developed extremely.

In a preferred embodiment of the present invention, the filter passes only the dissolved substance particles having sizes of not more than 10 μm.

The sample supplying nozzle

12

may be composed of a stainless steel pipe or a titanium pipe having a {fraction (1/16)} inch outer diameter and a 250 μm or below inside diameter.

The ion accelerating electrode part

2

has a first high vacuum chamber

20

and an accelerating electrode

21

. In FIGURE, the vacuum chamber

10

constituting the mass spectrometry interface

1

and the first high vacuum chamber

20

are united via the chamber wall

10

A of the vacuum chamber

20

.

Because of the unification of the above vacuum chamber, the ion accelerating electrode chamber part

2

has a laser beam- introducing window

22

to introduce a laser beam from the laser source

13

onto the rotation-translation drum

11

via the laser beam inlet

14

. Moreover, since a vacuum pump

23

such as a cryopump is positioned at the area denoted by a broken line in the first high vacuum chamber

20

, the interior of the chamber

20

is evacuated up to high vacuum degree.

In FIGURE, the laser beam inlet

14

is formed at the opposite side position of the chamber wall

10

A of the vacuum chamber

10

to the sample supplying nozzle

12

for the rotation-translation drum

11

. Thereby, the contamination in the ion accelerating electrode part

2

, adjacent to the laser beam inlet

14

, due to the liquid sample emitted from the sample supplying nozzle

12

can be prevented efficiently. Moreover, the ionized dissolved substance can be taken out efficiently, and thus, the mass spectrometry sensitivity can be enhanced.

Only if the above effects are attained, the laser beam inlet

14

may be formed at the upper side or the lower side of the chamber wall

10

A. However, if the laser beam inlet is situated at the above position, the prevention of the contamination and the enhancement of the mass spectrometry sensitivity can be performed at the most.

The mass spectrometry part

3

has a second high vacuum chamber

30

, a reflectron-reflective electrode

31

and a detector

32

. In the mass spectrometer depicted in FIGURE, the forefront tube

30

A of the second high vacuum chamber

30

is directly inserted into the first high vacuum chamber

20

, and thereby, the ionized dissolved substance which is accelerated at the accelerating electrode

21

is taken out efficiently.

The reflectron-reflective electrode

31

and the detector

32

are commercially available.

Moreover, a vacuum pump

33

such as a cryo pump is positioned at the area denoted by a broken line in the second high vacuum chamber

30

to evacuate the interior of the chamber.

Next, a mass spectrometry using the above mass spectrometer shown in FIGURE.

First, the interior of the vacuum chamber

10

in the mass spectrometry interface

1

is evacuated up to a given vacuum degree. Subsequently, the liquid sample is emitted for the rotation-translation drum

11

from the sample supplying nozzle

12

with rotating and translating the drum

11

. Just then, the liquid sample exhibits phase-transition to a mixture of gas and solid, and only the thus obtained dissolved substance of the liquid sample is stabilized as a solid spiral line on the drum

11

.

Then, a laser beam is irradiated onto the isolated substance from the laser source

13

via the laser beam introducing window

22

and the laser beam inlet

14

. In this time, the isolated substance is ionized and introduced into the ion accelerating electrode part

2

from the laser beam inlet

14

. Thereafter, the ionized substance is accelerated by the accelerating electrode

21

, and introduced into the mass spectrometry part

3

through the forefront tube

30

A of the second vacuum chamber

30

.

The ionized dissolved substance, which is accelerated as mentioned above, approaches to the reflectron-reflective electrode

31

and compensated in its kinetic energy fluctuation, and then, reaches the detector

32

.

The above operation is carried out continuously with rotating and translating the rotation-translating drum

11

. That is, the continuous irradiation of the laser beam enables the isolated substance to be detected continuously at high ionization, so that the detection sensitivity of the mass spectrometry can be enhanced. Moreover, since in this mass spectrometry, a sample which is apt to be chemically denaturalized is not employed and such a high detection sensitivity is attained, the mass spectrometry can be performed precisely.

Therefore, the above long time-continuous mass spectrometry for a liquid chromatograph, etc. can be carried out precisely.

Moreover, due to the small ionization efficiency of the isolated substance, the substance may not sometimes ionized effectively only by the laser beam irradiation, and thus, the detection sensitivity may not be enhanced effectively. In this case, the ionization of the light harvesting substance is developed by the ionization enhancing nozzle

15

, and thereafter, the solute substance on the layer of light harvesting substance is secondary ionized and analyzed in its mass.

Concretely, before the liquid sample is emitted from the sample supplying nozzle

12

, an optical absorption material is emitted for the rotation-translation drum

11

from the ionization enhancing nozzle

15

with rotating and translating the drum

11

, and then, an optical absorption layer made of the optical absorption material is formed on the drum

11

.

Subsequently, as mentioned above, the liquid sample is emitted for the rotation-translation drum

11

from the sample supplying nozzle

12

. In this case, the solute substance of the liquid sample is located at the surface area of the optical absorption layer. And, when the laser beam is irradiated onto the located solute substance, the ionization of the solute substance is developed indirectly through the location effect of the solute substance and the optical absorption effect of the optical absorption layer. As a result, the detection sensitivity of the mass spectrometry is developed from the increase of the ionization of the solute substance, and thus, the above advantages are attained.

Although the present invention was described in detail with reference to the above examples, this invention is not limited to the above disclosure and every kind of variation and modification may be made without departing from the scope of the present invention.

As mentioned above, according to the present invention, the ionization of the dissolved substance can be enhanced only by the laser beam irradiation without the addition of the above matrix reagent or the application of the high voltage. Therefore, the detection sensitivity of the mass spectrometer can be developed and thus, the long time-continuous mass spectrometry can be performed precisely.

Claims

1. A mass spectrometry interface comprising a vacuum chamber with a laser beam inlet, a rotation-translation drum installed in the vacuum chamber, said rotation-translation drum having a metallic surface and being capable of rotating and translating the surface of the drum, a sample supplying nozzle to emit and stabilize a liquid sample incorporating solute substance to be isolated and analyzed in its mass for and onto the metallic surface of the rotation-translation drum, and a laser source to irradiate a laser beam onto the dissolved substance from the laser beam inlet and to ionize the isolated substance.
2. A mass spectrometry interface as defined in claim 1, wherein the laser beam inlet is situated at the opposite position of the vacuum chamber to the sample supplying nozzle with the rotation-translation drum in therebetween.
3. A mass spectrometry interface as defined in claim 1, wherein the rotation-translation drum has a double structure composed of a shaft and a cylindrical titanium rim connected to the shaft.
4. A mass spectrometry interface as defined in claim 1, wherein the sample supplying nozzle has a heating cap at its forefront.
5. A mass spectrometry interface as defined in claim 1, wherein the sample supplying nozzle has a filter therein.
6. A mass spectrometry interface as defined in claim 1, further comprising a nozzle to enhance the ionization of the solute substance through the preliminary emission of an optical absorption material for the rotation-translation drum and thus the formation of an optical absorption layer made of the optical absorption material between the metal and the sample layers.
7. A mass spectrometer comprising a mass spectrometer interface as defined in claim 1, an ion accelerating electrode part and a mass spectrometry part.
8. A mass spectrometer as defined in claim 7, wherein the ion accelerating electrode part comprises a first high vacuum chamber and an accelerating electrode.
9. A mass spectrometer as defined in claim 7, wherein the mass spectrometry part comprises a second high vacuum chamber, a reflectron-reflective electrode and a detector.
10. A mass spectrometry method comprising the steps of:evacuating up to a given vacuum degree the interior of a vacuum chamber of a mass spectrometry interface constituting a mass spectrometer, emitting a liquid sample incorporating a dissolved substance to be analyzed in its mass to a rotation-translation drum from a sample supplying nozzle of the mass spectrometry interface and thereby, isolating the dissolved substance on the rotation-translation drum by rotating and translating the drum, and irradiating the isolated solute substance with a laser beam from a laser source of the mass spectrometry interface via a laser beam inlet formed at the vacuum chamber and thereby, ionizing the solute substance.
11. A mass spectrometry as defined in claim 10, further comprising the step of emitting an optical absorption material for the rotation-translation drum from a nozzle to enhance the ionization of the dissolved substance and then, forming an optical absorption layer made of the optical absorption material thereon with rotating and translating the rotation-translation drum before the liquid sample is emitted for the rotation-translation drum and the dissolved substance of the liquid sample is isolated thereon.

Priority Claims (1)

Number	Date	Country	Kind
2000-242002	Aug 2000	JP

US Referenced Citations (2)

Number	Name	Date	Kind
4740298	Andresen et al.	Apr 1988	A
6175112	Karger et al.	Jan 2001	B1

Foreign Referenced Citations (4)

Number	Date	Country
60-146438	Aug 1985	JP
9-326243	Dec 1997	JP
2002-502543	Jan 2002	JP
9853308	Nov 1998	WO

Non-Patent Literature Citations (8)

Entry
E. D. Hardin et al, Anal. Chem. 1981, 53, 1492-1497.*
E. D. Hardin et al, Anal. Chem. 1984, 56, 2-7.*
T. P. Fan et al, Anal. Chem. 1984, 56, 1870-1876.*
G. M. Kresbach et al, J. Chromatog. 1987, 394, 89-100.*
E. R. Verheij et al, J. Chromatog. 1989, 474, 275-283.*
X. Fei et al, Anal. Chem. 1996, 68, 1143-1147.*
H. Zhang et al, J. Mass Spectrom. 1996, 31, 1039-1046.*
J. L. Dwyer ACS Symp. Ser. 1999, 731, 84-94.

Mass spectrometry interface, a mass spectrometer and a mass spectrometry

Information

Patent Number

Date Filed

Date Issued

Inventors

Original Assignees

Examiners

Agents

CPC

US Classifications

Field of Search

US

International Classifications