Microcell And Microcell Holder

Description

BRIEF DESCRIPTION OF THE DRAWINGS

FIGS. 1A to 1E are views showing an outline structure of a microcell according to an embodiment of the present invention.

FIG. 2 is a view showing an outline structure of a microcell holder holding the microcell of the embodiment of the present invention.

FIG. 3A shows the microcell holder holding the microcell of the embodiment of the present invention, viewed from a direction orthogonal to an optical axis.

FIG. 3B is an enlarged view of a cell switching knob of the microcell holder shown in FIG. 3A.

FIG. 3C shows the microcell holder shown in FIG. 3A, viewed from the direction of the optical axis.

FIGS. 4A to 4C are views showing a cell attaching-and-detaching mechanism suitable for the microcell holder of the embodiment of the present invention.

FIGS. 5A and 5B are views showing a cell positioner suitable for the microcell holder of the embodiment of the present invention.

FIGS. 6A and 6B show a modified example of the cell positioner shown in FIG. 5.

FIG. 7 is a view showing a mask position adjuster suitable for the microcell holder of the embodiment of the present invention.

FIGS. 8A to 8D are views showing a microcell using mechanical contact according to another embodiment of the present invention.

FIG. 9 is a view showing an outline structure of a translation microcell according to another embodiment of the present invention.

DESCRIPTION OF THE PREFERRED EMBODIMENTS

Preferred embodiments of the present invention will be described below with reference to the drawings.

FIGS. 1A to 1E show an outline structure of a microcell according to an embodiment of the present invention. FIG. 1A shows the microcell viewed from a light entry side; FIG. 1B shows a vertical cross-sectional view of the microcell; FIG. 1C shows an enlarged view of a main part of the microcell; FIG. 1D shows an enlarged view of a main part of a cell chamber; and FIG. 1E shows the microcell viewed from above.

The present invention is characterized by the configuration of multiple cells and by reduction in the amount of the liquid sample required to conduct appropriate analysis, so that a very small amount of the liquid sample can be efficiently analyzed. The microcell according to the present invention is structured as described below.

A microcell 10 shown in FIGS. 1A to 1E is circular and includes a circular plate (plate spacer) 12 and window plates 14.

The circular plate 12 is made of a solvent-resistant material (such as a resin). The circular plate 12 has a plurality of small circular holes (small holes) 24 each having notches 22 whose width increases toward a sample injection opening 20 in an outer wall. The small circular holes 24 are disposed in such a manner that the centers of the small circular holes 24 are positioned on a circumference near the rim of the circular plate 12 at regular intervals.

The window plates 14 are doughnut-shaped plates made of a material that passes measuring light L (such as a fused silica plate). The window plates 14 are disposed to block or cover the small circular holes 24 of the circular plate 12 from both the light entry side and the light exit side, facing each other on either side of the circular plate 12.

In this embodiment, the circular plate 12 and the window plates 14 are bonded (welded) to each other so that the liquid sample does not leak out. The spaces enclosed by the small circular holes 24 of the circular plate 12 and the window plates 14 are cell chambers 30 for containing the liquid sample.

In this embodiment, the microcell 10 has eight small circular holes 24 in the circular plate 12, and the small circular holes 24 covered with the window plates 14 form eight cell chambers 30.

The diameter of the small circular holes 24 and the thickness of the circular plate 12 of the microcell 10 are determined by the amount of the liquid sample. The internal dimension D₁of a joining part 25 between the notches 22 and the small circular hole 24 of the microcell 10 is smaller than the internal diameter D₂of the small circular hole 24.

The microcell 10 of this embodiment further includes an entry-side outer frame 40 and an exit-side outer frame 42. The entry-side outer frame 40 and the exit-side outer frame 42 are disposed to face each other on either side of the circular plate 12.

The microcell 10 of this embodiment is roughly structured as described above, and its advantages will be described next. The microcell 10 of the embodiment can provide a cell chamber 30 having such a capacity that a liquid sample available even in a very small amount can be appropriately analyzed, by adjusting the thickness of the circular plate 12 or the diameter D₂of the small circular hole 24 in accordance with the amount of the liquid sample. For instance, when the circular plate 12 has a thickness of 1 mm and the small circular hole 24 has a diameter D₂of 2 mm, the cell chamber 30 has a capacity of 3 microliters.

A plurality of cell chambers 30 can be provided easily and reliably in this embodiment, so that multiple microcells 10 can be configured easily and reliably. In the embodiment, since the liquid sample is held in each cell chamber 30 by surface tension, the multiple microcells 10 can be provided with great ease and reliability.

The circular plate 12 and the window plates 14 bonded (welded) to each other in this embodiment are very effective in preventing liquid leakage, in comparison with mechanical close contact made by a window retainer, a screw, or the like. The cell chambers can thus hold the liquid sample reliably.

The advantages will be described in detail. The liquid sample to be analyzed is put into the microcell 10 through the sample injection opening 20 by means of a microsyringe or the like.

The microcell 10 has the small circular holes 24 near the rim of the circular plate 12, and the small circular holes 24 each have the notches 22 whose width increases toward the sample injection opening 20 from the small circular hole 24.

Because the width or the internal dimension of the notches 22 is maximum at the sample injection opening 20, a tip of a micropipette or the like can be easily put into or taken out of the sample injection opening 20, and the liquid sample can be put into the cell chamber 30 efficiently.

Because the small circular holes 24 and the notches 22 are disposed on the circumference near the rim of the circular plate 12, the distance between the outer wall of the cell and the cell chamber is shorter than that in general V-shaped microcells. Accordingly, the liquid sample can be put into the cell chambers 30 more accurately with ease, providing more efficient liquid-sample injection.

With the width or internal diameter D₁of the notches 22 minimized in the joining part 25 or the boundary of the small circular hole 24, the cell is designed to securely hold the liquid sample put into the cell chamber 30 by surface tension, without a lid.

In the microcell 10, the internal diameter D₁of the joining part 25 between the notches 22 and the small circular hole 24 is smaller than the internal diameter D₂of the small circular hole 24, so that the liquid sample is held in the cell chamber 30 by surface tension.

Accordingly, in comparison with general cells requiring a lid, this embodiment allows the liquid sample to be put into the cell chambers 30 more efficiently and allows multiple microcells to be configured with ease.

The microcell 10 of the embodiment, configured as described above, allows samples available even in a very small amount to be measured successively with reliability, which will result in a leap in analysis efficiency.

After the liquid sample is prepared, the microcell 10 is mounted in an analysis apparatus, where the liquid sample in each cell chamber is analyzed. In this embodiment, it is preferable that a microcell holder, which will be described below, be used to conduct successive measurement with the microcell 10 appropriately and efficiently.

FIG. 2 shows a microcell holder 50 holding the microcell 10 of the embodiment. The figure shows the microcell holder viewed from above.

The microcell holder 50 shown in the figure includes a cell table 52 and a cell switcher 54.

The cell table 52 is provided on a base 58 of a sample chamber 56 in the main body of an ultraviolet-visible spectrophotometer, or an analysis apparatus.

The cell switcher 54 is provided on the cell table 52 and holds the microcell 10 in such a manner that it can be rotated to place a desired cell chamber 30 on an optical path X in the sample chamber 56.

The cell switcher 54 includes a cell support 59, an output-side cell switching shaft 60, an output-side cell switching shaft bearing 62, an output-side bevel gear 64, an input-side bevel gear 66, an input-side cell switching shaft 68, an input-side cell switching shaft bearing 70, and a cell switching knob 72, as holder and rotator of the present invention.

The cell support 59 supports the microcell 10 rotatably in such a manner that the optical axis X is orthogonal to the window plate 14.

The output-side cell switching shaft 60 rotates the cell support 59 about a line parallel to the optical axis X. The output-side cell switching shaft bearing 62 supports the output-side cell switching shaft 60 rotatably.

The input-side cell switching shaft 68 rotates about a line orthogonal to the optical axis X.

The input-side cell switching shaft bearing 70 supports the input-side cell switching shaft 68 rotatably.

The cell switching knob 72 rotates the input-side cell switching shaft 68.

The microcell holder 50 of the embodiment includes a lens 80 for focusing the measuring light L coming from a previous stage onto the liquid sample in the cell chamber 30, a mask 81 for narrowing the measuring light L, and a lens 82 for collimating the measuring light L passing through the liquid sample in the cell chamber 30.

In this embodiment, a reference microcell holder 86 is provided to hold a reference microcell to be compared with the microcell 10.

The microcell holder 50 of the embodiment is configured roughly as described above, and its advantages will be described next. When successive measurement is conducted with the microcell 10, the microcell 10 is mounted in the microcell holder 50; the measuring light L is applied to the liquid sample in a desired cell chamber 30 in the ultraviolet-visible spectrophotometer; and the light passing through the sample is measured.

In this embodiment, the cell switcher 54 allows desired cell chambers 30 to be placed successively on the optical path X with ease and reliability, so that successive measurement of the liquid samples in the cell chambers 30 of the microcell 10 can be conducted efficiently and reliably.

The advantages will be described in detail. In the present embodiment, the microcell 10 containing the liquid sample is placed in the microcell holder 50 in the sample chamber 56 in such a manner that the measuring light L passes through a desired cell window, or an area of the window plates 14 corresponding to a desired cell chamber 30, at a right angle.

After the microcell is placed in the microcell holder 50, the measuring light L is focused by the lens 80, narrowed by the mask 81, and incident on the liquid sample in the desired cell chamber 30. The light passing through the liquid sample in the cell chamber 30 is substantially collimated to parallel rays L by the lens 82, guided into a subsequent stage, and used for analysis.

In this embodiment, since the measuring light L is incident on the liquid sample through the window plate 14, and the transmitted light L is obtained, the usage rate of the measuring light is higher in comparison with measurement using an optical fiber. Accordingly, even a small amount of a liquid sample can be appropriately analyzed.

In the present embodiment, the mask 81 is disposed just in front of the microcell 10. The mask 81 narrows the measuring light L coming from the previous stage and directs the light into a desired cell chamber 30 of the microcell 10. Accordingly, this embodiment allows the measuring light L to be reliably directed into the desired cell chamber 30 of the microcell 10.

In the present embodiment, the cell switcher 54 makes it possible to measure the liquid samples in the cell chambers 30 successively by rotating the microcell 10. With the microcell 10 placed in the microcell holder 50 in such a manner that the measuring light L passes through the cell chamber 30 at a right angle, as shown in FIG. 3A, the operator turns the cell switching knob 72, shown in FIG. 3B, to rotate the microcell 10, as shown in FIG. 3C. This simple operation reliably and easily places the desired cell chambers 30 successively on the optical path X in the sample chamber.

In this embodiment, the cell switcher 54 allows the desired cell chambers 30 of the microcell 10 to be placed successively on the optical path X with ease and reliability, so that successive measurement of the liquid samples in the cell chambers 30 of the microcell 10 can be conducted appropriately and efficiently.

As shown in FIG. 3B, numbers are marked on the cell switching knob 72, so that the cell chamber 30 placed on the optical path X can be identified. The operator can correctly identify the cell chamber 30 currently placed on the optical path X by this number. Therefore, the desired cell chamber 30 can be placed on the optical path and measured with ease and reliability.

After the measurement, the liquid samples in the cell chambers 30 can be easily collected by a microsyringe or the like. Then, the cell chambers 30 can be cleaned by water or the like.

As described above, the microcell holder 50 of the present embodiment includes the cell switcher 54. Accordingly, multiple cell chambers 30 of the microcell 10 can be successively placed on the optical path X easily and appropriately in this embodiment. With the microcell 10, even a very small amount of a sample can be analyzed appropriately and efficiently. Moreover, successive measurement can be conducted appropriately and efficiently with the cell chambers 30 of the microcell 10. Therefore, this embodiment results in a leap in analysis efficiency of a small amount of a sample of about a few microliters, which was previously very difficult.

In this embodiment, it is also very important for reliable and efficient analysis that the microcell be capable of being placed in the microcell holder easily and reliably.

Accordingly, it is very preferable that a cell attaching-and-detaching mechanism, shown in FIG. 4, be further provided in this embodiment. FIG. 4A shows a vertical cross-sectional view of the microcell and a part of the microcell holder; FIG. 4B shows the cell attaching-and-detaching mechanism (on the microcell side) viewed from the entry side; and FIG. 4C shows the cell attaching-and-detaching mechanism (on the microcell-holder side) viewed from the exit side.

A cell attaching-and-detaching mechanism 90 shown in the figure includes a cell support 59, a positioning pin 92, and an indentation 94.

The cell support 59 is disposed on the side of the microcell holder and rotates with the output-side cell switching shaft 60 to support the microcell 10.

The positioning pin 92 is disposed on the entry-side outer frame 40 of the microcell 10, and the indentation 94 is provided in the cell support 59.

The positioning pin 92 and the indentation 94 are used to position the microcell 10 and the microcell holder 50.

The microcell 10 and the microcell holder 50 of the present embodiment has the positioning pin 92 and the indentation 94. When spectral analysis is conducted, this embodiment allows the microcell 10 to be placed in a predetermined position of the microcell holder 50 easily and accurately just by placing the microcell 10 on the cell support 59 of the microcell holder 50 in such a manner that the positioning pin 92 fits in the indentation 94. The present embodiment improves the positioning repeatability of the microcell 10 on the microcell holder 50, so that successive measurements with multiple cell chambers 30 of the microcell 10 can be conducted with great ease and reliability.

In the embodiment, it is also preferable for efficient analysis that the entry-side outer frame 40 of the microcell 10 and the cell support 59 of the microcell holder 50 (holder and rotator) contain a magnet 96 in their mounting parts so as to easily and detachably mount the microcell 10 on the cell support 59 of the microcell holder 50 by a magnetic force of the magnet 96.

It is strongly preferable in this embodiment that the microcell 10 be detachable from the side opposite to the mask 81. If the microcell 10 were detachable from the mask side, the mask 81 just in front of the microcell 10 would obstruct the attaching and detaching of the microcell 10.

If the mask 81 is disposed so as to keep a certain distance from the microcell 10, so that the microcell 10 can be easily attached or detached, the effect of the mask 81 of the present invention, namely, the effect of narrowing the measuring light L coming from the previous stage and directing the light into a desired cell chamber 30 accurately, might not be sufficiently provided.

In addition, it is very important in this embodiment that a cell positioner for rotating the microcell 10 to place a desired cell chamber 30 accurately on the optical path X be provided to conduct the analysis more accurately and efficiently.

According to the present invention, it is preferable that the cell positioner be provided for the microcell 11 or a portion where the microcell 10 is integrated. A strongly preferable position on the microcell 10 or on the portion where the microcells 10 is integrated is on the circular face of the microcell 10 or on the circumferential wall (side wall) of the microcell 10.

FIGS. 5A and 5B show an outline structure of the cell positioner. FIG. 5A shows a vertical cross-sectional view of an area in the vicinity of the cell positioner viewed from a side; FIG. 5B shows the microcell side of the cell positioner viewed from the previous stage.

A cell positioner 98 shown in FIG. 5A includes a fixed member 99a, a movable member 99b, indentations 100, a spring 102, a screw 103, and a ball 104.

The fixed member 99a is secured to the microcell holder 50 and faces the circular face of the microcell 10 or the movable member 99b.

The movable member 99b is provided on the circular face of the microcell 10 and rotates with respect to the fixed member 99a. The movable member 99b has as many indentations 100 as the cell chambers 30 of the microcell 10. In this embodiment, eight indentations 100 are provided on the circular face of the movable member 99b at regular intervals.

The ball 104 fits in the indentation 100 and is held by the screw 103 provided on the fixed member 99a, and is pressed toward the indentation 100 by the spring 102.

When the operator rotates the cell switching knob 72, the movable member 99b provided on the microcell 10 rotates with respect to the fixed member 99a of the cell positioner 98. Each time it rotates by a prescribed angle, that is, each time a cell chamber 30 is placed on the optical path, the ball 104 engages with the indentation 100. When this engagement occurs, the operator can judge that the cell chamber 30 is accurately placed on the optical path.

The embodiment makes it easy and reliable to successively position a plurality of cell chambers 30 accurately on the optical path. Because the positioning repeatability of the cell chambers 30 increases, successive measurements with multiple cell chambers 30 of the microcell 10 can be conducted easily and appropriately.

In this embodiment, the positioner 98 is preferably provided for the microcell 10 or a portion where the microcell 10 is integrated, that is, the movable member 99b. This can more reliably avoid the effect of a positioning error because of a movement error of a transfer shaft or the like, in comparison with a case where the positioner 98 is disposed separately from the microcell 10. Accordingly the cell chambers 30 can be positioned with higher reliability.

FIGS. 6A and 6B show a modified example of the cell positioner shown in FIG. 5. FIG. 6A shows the positioner viewed from a side; and FIG. 6B shows a vertical cross-sectional view of the positioner viewed from the side of the circular face.

A cell positioner 98 shown in FIG. 6A is disposed to face the side wall of the microcell 10.

A fixed member 99a secured to the microcell holder 50 is disposed to face an upper part of the side wall of the microcell 10.

Indentations 100 are provided in the circumferential wall (side wall) of a movable member 99b at regular intervals.

The cell positioner 98 structured as shown in FIG. 6A has the same advantages as the cell positioner 98 shown in FIG. 5A.

In addition, it is very important in this embodiment that the position of the mask 81 disposed just in front of the microcell 10 be adjusted to direct the measuring light into a desired cell chamber 30 of the microcell 10 with higher reliability.

For example, the internal diameter of the cell chamber 30 is as very small as, for example, about 1.6 mm, and the diameter of an aperture 81a of the mask 81 is also as very small as about 1.0 mm. Accordingly, it is preferable that mask position adjuster 108 be provided to adjust the position of the optical axis of the mask 81.

As shown in FIG. 7, the mask position adjuster 108 can move the position of the optical axis of the mask 81, or the position of the aperture 81a in a desired manner in a plane orthogonal to the optical path X in the ultraviolet-visible spectrophotometer, in horizontal directions (indicated by arrows “i” in the figure) and vertical directions (indicated by arrows “j” in the figure) in this embodiment.

The position of the optical axis of the mask 81 can be adjusted with the mask position adjuster 108 described above, so that the measuring light L can be directed into the very small cell chamber 30 of the microcell 10 with higher reliability.

The microcell 10 having eight cell chambers 30 has been described above, but the present invention can be applied to any other number of cell chambers.

In the configuration described above, the cell chamber 30 to be placed on the optical path X is switched by the cell switching knob 72, which is manually rotated by the operator from the outside of the sample chamber 56. The cell chamber 30 can also be switched automatically. For example, a driving force may be transferred from a motor to the input-side cell switching shaft 68 to rotate the input-side cell switching shaft 68 by computer control, so that the cell chamber 30 placed on the optical path X is switched automatically.

In the configuration described above, it is strongly preferred that the plate spacer and the window plates be bonded to each other. The cell formed by bonding the plate spacer and the window plates to each other is much more effective in preventing liquid leakage than that formed by mechanical close contact using a window retainer, a screw, or the like. The cell chamber can hold the liquid sample reliably.

However, the circular plate (plate spacer) 12 and the window plates 14 of the microcell 10 may also be brought into close contact with each other by a mechanical method using a window retainer, a screw, or the like.

FIGS. 8A to 8D show a modified example of the microcell of the embodiment. FIG. 8A shows the microcell viewed from the light entry side; FIG. 8B shows a vertical cross-sectional view of the microcell; FIG. 8C shows an enlarged view of a main part of the microcell; and FIG. 8D shows the microcell viewed from above.

Although doughnut-shaped window plates are used as the window plates 14 in the configuration described above, a plurality of pairs of circular window plates 14 are used in FIGS. 8A to 8D. These pairs of circular window plates 14 are disposed at corresponding cell chambers 30.

The microcell 10 shown in FIGS. 8A to 8D includes window retainers 16. The window retainers 16 are made of a plate of rigid metal or the like. The window retainers 16 are disposed to face each other on either side of the window plates 14 in such a manner that the window plates 14 are tightened toward the circular plate 12 with a screw or the like. The circular plate 12 and the window plates 14 are brought into close contact with each other, so that the liquid sample will not leak. The window retainers 16 have light-passing holes 28 for passing the measuring light 26 through the window plates 14.

In the embodiment, small circular holes 24 closed off by the window plates 14 form eight cell chambers 30.

In the embodiment, an entry-side outer frame 40 and an exit-side outer frame 42 are disposed to face each other on either side of the window retainers 16.

It is strongly preferable that the microcell 10 have a plurality of cell chambers 30 disposed on a circumference of the circular plate 12 at regular intervals, as described above. It is also preferable that a plurality of cell chambers 30 be disposed in a line in the longitudinal direction on a long plate (plate spacer) 110 as shown in FIG. 9.

In this case, it is preferred that a microcell holder use, instead of the rotator, a translator 112 for moving a microcell 10 linearly in a direction (indicated by arrows “I” in the figure) orthogonal to the optical axis, as a cell switcher for switching the cell chamber 30 placed on the optical path X.

Although the microcell having the window plates and the spacer bonded (welded) to each other is strongly preferred, as described above, a cell can also be configured with window plates and a spacer brought into close contact with each other by a cell retainer. A liquid sample is reliably held in a cell chamber 30 by surface tension without a lid, as in the microcell having the window plates and the spacer bonded (welded) to each other, so that multiple cells can be easily configured.

Claims

1. A microcell used in analysis of very small amounts of liquid samples, the microcell comprising: a plate spacer having a plurality of small holes with notches widening toward sample injection openings in a side wall; andwindow plates made of a material passing measuring light, disposed to face each other on either side of the spacer to cover the plurality of small holes from the front and the back;wherein spaces formed by the plurality of small holes of the spacer and the window plates serve as a plurality of cell chambers for containing the liquid samples; anda dimension of the plurality of small holes and the thickness of the spacer are determined in accordance with the amounts of the liquid samples, and a dimension of parts joining the notches and the plurality of small holes is smaller than the dimension of the plurality of small holes.
2. A microcell according to claim 1, further comprising window retainers disposed on either side of the window plates for bringing the spacer and the window plates into close mechanical contact with each other.
3. A microcell according to claim 1, wherein the plate spacer and the window plates are welded to each other.
4. A microcell holder for holding a microcell according to claim 1 on an optical path in an analysis apparatus, the microcell holder comprising: a cell switcher for holding the microcell in such a movable manner that a desired one of the plurality of cell chambers is placed on the optical path in the analysis apparatus.
5. A microcell holder for holding a microcell according to claim 2 on an optical path in an analysis apparatus, the microcell holder comprising: a cell switcher for holding the microcell in such a movable manner that a desired one of the plurality of cell chambers is placed on the optical path in the analysis apparatus.
6. A microcell holder for holding a microcell according to claim 3 on an optical path in an analysis apparatus, the microcell holder comprising: a cell switcher for holding the microcell in such a movable manner that a desired one of the plurality of cell chambers is placed on the optical path in the analysis apparatus.
7. A microcell holder according to claim 4, wherein the cell switcher holds the microcell, which is substantially circular; andthe cell switcher comprises:holder for holding the microcell in such a rotatable manner that the microcell is rotated to place the desired one of the plurality of cell chambers on the optical path in the analysis apparatus; androtator for rotating the holder for holding the microcell to place the desired one of the plurality of cell chambers on the optical path in the analysis apparatus.
8. A microcell holder according to claim 5, wherein the cell switcher holds the microcell, which is substantially circular; andthe cell switcher comprises:holder for holding the microcell in such a rotatable manner that the microcell is rotated to place the desired one of the plurality of cell chambers on the optical path in the analysis apparatus; androtator for rotating the holder for holding the microcell to place the desired one of the plurality of cell chambers on the optical path in the analysis apparatus.
9. A microcell holder according to claim 6, wherein the cell switcher holds the microcell, which is substantially circular; andthe cell switcher comprises:holder for holding the microcell in such a rotatable manner that the microcell is rotated to place the desired one of the plurality of cell chambers on the optical path in the analysis apparatus; androtator for rotating the holder for holding the microcell to place the desired one of the plurality of cell chambers on the optical path in the analysis apparatus.
10. A microcell holder according to claim 4, further comprising a mask disposed just in front of the microcell, for narrowing measuring light coming from a previous stage and directing the light into a liquid sample contained in the desired one of the plurality of cell chambers.
11. A microcell holder according to claim 10, wherein the microcell is detachable from the side opposite to the mask.
12. A microcell holder according to claim 10, further comprising mask position adjuster for adjusting, in a desired manner, the position of the optical axis of the mask with respect to the optical path in the analysis apparatus in a plane orthogonal to the optical path.

Priority Claims (1)

Number	Date	Country	Kind
2006-156843	Jun 2006	JP	national

Microcell And Microcell Holder

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CPC

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Abstract

Description

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Priority Claims (1)