JP2023022846A - Sample preparation method, freeze pressurization device, and observation method - Google Patents

Sample preparation method, freeze pressurization device, and observation method Download PDF

Info

Publication number
JP2023022846A
JP2023022846A JP2019211101A JP2019211101A JP2023022846A JP 2023022846 A JP2023022846 A JP 2023022846A JP 2019211101 A JP2019211101 A JP 2019211101A JP 2019211101 A JP2019211101 A JP 2019211101A JP 2023022846 A JP2023022846 A JP 2023022846A
Authority
JP
Japan
Prior art keywords
sample preparation
opening
housing member
fixing
observed
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Pending
Application number
JP2019211101A
Other languages
Japanese (ja)
Inventor
昭夫 清水
Akio Shimizu
大史 佐谷
Hiroshi Satani
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
Nichirei Corp
Soka University
Original Assignee
Nichirei Corp
Soka University
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Nichirei Corp, Soka University filed Critical Nichirei Corp
Priority to JP2019211101A priority Critical patent/JP2023022846A/en
Priority to JP2021558232A priority patent/JPWO2021100396A1/ja
Priority to PCT/JP2020/039620 priority patent/WO2021100396A1/en
Publication of JP2023022846A publication Critical patent/JP2023022846A/en
Pending legal-status Critical Current

Links

Images

Classifications

    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N1/00Sampling; Preparing specimens for investigation
    • G01N1/28Preparing specimens for investigation including physical details of (bio-)chemical methods covered elsewhere, e.g. G01N33/50, C12Q
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N1/00Sampling; Preparing specimens for investigation
    • G01N1/28Preparing specimens for investigation including physical details of (bio-)chemical methods covered elsewhere, e.g. G01N33/50, C12Q
    • G01N1/42Low-temperature sample treatment, e.g. cryofixation

Landscapes

  • Physics & Mathematics (AREA)
  • Health & Medical Sciences (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Chemical & Material Sciences (AREA)
  • Analytical Chemistry (AREA)
  • Biochemistry (AREA)
  • General Health & Medical Sciences (AREA)
  • General Physics & Mathematics (AREA)
  • Immunology (AREA)
  • Pathology (AREA)
  • Sampling And Sample Adjustment (AREA)

Abstract

To provide a sample preparation method for suppressing formation of an ice crystal, a freeze pressurization device and an observation method.SOLUTION: A sample preparation method includes: a step for filling a space inside of a sample preparation device 10 comprising a first housing member 11a and a second housing member 11b having a cavity unit and an opening unit with one surface of the cavity unit opened with an object to be observed and water; a step of fixing the opening of the first housing member 11a and the opening of the second housing member 11b together; a step of cooling the sample preparation device 10; and a step of dividing the object to be observed frozen by the step of cooling, by separating the first housing member 11a and the second housing member 11b.SELECTED DRAWING: Figure 4

Description

特許法第30条第2項適用申請有り 令和1年10月23日、日本高圧力学会主催、第60回高圧討論会にて発表。 令和1年11月21日、イオン液体研究会主催、第10回イオン液体討論会にて発表。Applied for the application of Article 30, Paragraph 2 of the Patent Law Presented at the 60th High Pressure Symposium hosted by the High Pressure Society of Japan on October 23, 2019. Presented at the 10th Ionic Liquid Symposium hosted by the Ionic Liquid Research Group on November 21, 2019.

本発明は、試料作製方法、凍結加圧装置および観察方法に関する。 TECHNICAL FIELD The present invention relates to a sample preparation method, a freezing pressurization device, and an observation method.

食品、植物、微小生物、細胞などといった水分含有量の多い物質を被観察物として顕微鏡で観察する場合において、当該被観察物を凍結させて、切断することで、観察用の試料を作製する、凍結割断試料作製技術が知られている(例えば、特許文献1など)。 When observing a substance with a high water content such as food, plants, micro-organisms, cells, etc. as an object to be observed with a microscope, the object to be observed is frozen and cut to prepare a sample for observation. A freeze-fracture sample preparation technique is known (for example, Patent Document 1, etc.).

しかしながら、被観察物に含まれる水分が凍結する際に氷晶が生成され、被観察物が破壊されるため、適切な観察ができないという問題があった。このような被観察物の破壊を抑制するため、有機溶媒などによって氷晶の生成を抑制する方法なども提案されているが、有機溶媒が被観察物に影響を及ぼすことがあり、やはり適切な観察には向かなかった。 However, when the water contained in the object to be observed freezes, ice crystals are generated and the object to be observed is destroyed, so there is a problem that proper observation cannot be performed. In order to suppress such destruction of the observed object, a method of suppressing the formation of ice crystals by using an organic solvent or the like has been proposed, but the organic solvent may affect the observed object. I didn't go to observe.

この点につき、非特許文献1や特許文献2などには、氷晶の生成を抑制する凍結技術が開示されている。ここで、非特許文献1に開示されている走査型電子顕微鏡(SEM)での観察用の試料を作製する方法について、図10を以て説明する。図10は、従来技術における観察用試料の作製の概略を示す図である。 In this regard, Non-Patent Document 1, Patent Document 2, and the like disclose freezing techniques for suppressing the formation of ice crystals. Here, a method for producing a sample for observation with a scanning electron microscope (SEM) disclosed in Non-Patent Document 1 will be described with reference to FIG. FIG. 10 is a diagram showing an outline of preparation of an observation sample in the prior art.

非特許文献1に記載されている従来技術では、図10(a)に示すような平板型試料作製装置50を用いて、凍結割断試料を作製する。従来技術における平板型試料作製装置50は、図10(b)に示すように、2つの平板型収容部材51a,51bに分割可能に構成される。平板型収容部材51a,51bは、上部が開放された窪みを有し、2つを連結することで、図10(a)のような試料作製領域が形成される。 In the conventional technique described in Non-Patent Document 1, a freeze-fractured sample is prepared using a plate-type sample preparing apparatus 50 as shown in FIG. 10(a). As shown in FIG. 10(b), the conventional plate-type specimen preparation apparatus 50 is configured to be divisible into two plate-type housing members 51a and 51b. The flat-plate storage members 51a and 51b have recesses with open tops, and by connecting the two, a sample preparation area as shown in FIG. 10(a) is formed.

図10(c)~(e)は、凍結割断試料作製方法の各工程を示している。まず、図10(c)のように、平板型試料作製装置50の窪み部分に被観察物と水を入れて、窪み部分を水で満たす。このとき、観察対象となる部位が、平板型収容部材51a,51bの境界に配置されるように、被観察物を配置する。 FIGS. 10(c)-(e) show each step of the freeze-fracture sample preparation method. First, as shown in FIG. 10(c), an object to be observed and water are placed in the hollow portion of the plate-type sample preparation apparatus 50 to fill the hollow portion with water. At this time, the object to be observed is arranged so that the site to be observed is arranged at the boundary between the flat plate-shaped housing members 51a and 51b.

その後、図10(d)に示すように、平板型試料作製装置50を冷却し、被観察物や水を凍結させる。平板型試料作製装置50を冷却する方法としては、冷却した金属ブロックを平板型試料作製装置50に当接させる方法が挙げられる。このとき、平板型試料作製装置50内の水は、外側の部分から凍結し、未凍結の水と被観察物とを内包しながらさらに冷却が進む。したがって、水や被観察物の水分が凍結する際に、体積の膨張が押さえ付けられ、氷晶の生成が抑制される。 After that, as shown in FIG. 10(d), the plate-type specimen preparation apparatus 50 is cooled to freeze the object to be observed and water. As a method for cooling the plate-shaped sample preparation device 50, there is a method of bringing a cooled metal block into contact with the plate-shaped sample preparation device 50. FIG. At this time, the water in the plate-type specimen preparation apparatus 50 freezes from the outer portion, and cooling proceeds further while unfrozen water and the object to be observed are included. Therefore, when the water or the moisture content of the object to be observed freezes, the volume expansion is suppressed, and the formation of ice crystals is suppressed.

平板型試料作製装置50の内容物を凍結させたあと、図10(e)に示すように、平板型収容部材51a,51bを分割する。平板型収容部材51a,51bは、窪み部分のうち、他方の平板型収容部材51と連結する箇所が細くなっていることから、平板型収容部材51を分割する際に被観察物が割断しやすい構造となっている。このようにして割断された被観察物は、真空乾燥後、オスミウムでコーティングされ、顕微鏡観察用の試料となる。 After freezing the contents of the plate-shaped sample preparation device 50, the plate-shaped storage members 51a and 51b are divided as shown in FIG. 10(e). In the flat plate-shaped storage members 51a and 51b, since the part of the recessed portion that is connected to the other flat-plate storage member 51 is narrow, the object to be observed is easily broken when the flat-plate storage member 51 is divided. It has a structure. The object to be observed cut in this way is vacuum-dried and then coated with osmium to form a sample for microscopic observation.

図10を以て説明した従来技術のように、凍結時に加圧することで氷晶の生成を抑制した試料を作製することができる。しかしながら、非特許文献1などの従来技術においては、冷却速度が10K/sの急速な冷却が必要であり、また、1mm以下(0.06ミリリットル程度)の小さな被観察物でしか、試料を作製することができなかった。 As in the prior art described with reference to FIG. 10, it is possible to prepare a sample in which the formation of ice crystals is suppressed by applying pressure when frozen. However, in the prior art such as Non-Patent Document 1, rapid cooling at a cooling rate of 10 K / s is required, and only small objects of 1 mm or less (about 0.06 ml) can be used to prepare samples. couldn't.

そのため、氷晶の生成を抑制する凍結割断試料作製技術において、さらなる利便性の向上が求められていた。 Therefore, there has been a demand for further improvements in the convenience of freeze-fracture specimen preparation techniques that suppress the formation of ice crystals.

本発明は、上記従来技術における課題に鑑みてなされたものであり、氷晶の生成を抑制する試料作製方法、凍結加圧装置および観察方法を提供することを目的とする。 SUMMARY OF THE INVENTION It is an object of the present invention to provide a sample preparation method, a freezing pressurization apparatus, and an observation method that suppress the formation of ice crystals.

すなわち、本発明によれば、
空洞部と、前記空洞部の1つの面が開口した開口部とを有する第1の部材および第2の部材からなる試料作製装置の内部の空間に、被観察物および水を入れて、前記空間に充填する工程と、
前記第1の部材の開口部と、前記第2の部材の開口部とを合わせて固定する工程と、
前記試料作製装置を冷却する工程と、
前記第1の部材および前記第2の部材を分離して、前記冷却する工程によって凍結した前記被観察物を割断する工程と
を含む、試料作製方法が提供される。 That is, according to the present invention,
An object to be observed and water are put into a space inside a sample preparation device comprising a first member and a second member having a hollow portion and an opening with one side of the hollow portion open, and the space is filled with water. filling into
aligning and fixing the opening of the first member and the opening of the second member;
a step of cooling the sample preparation device;
and a step of separating the first member and the second member and cutting the frozen observation object by the cooling step.

本発明によれば、氷晶の生成を抑制する試料作製方法、凍結加圧装置および観察方法が提供できる。 According to the present invention, it is possible to provide a sample preparation method, a freezing pressurization apparatus, and an observation method that suppress the formation of ice crystals.

本実施形態の試料作製装置の構造を示す斜視図。1 is a perspective view showing the structure of a sample preparation apparatus according to this embodiment; FIG. 本実施形態の試料作製装置を構成する収容部材の構造を示す図。FIG. 2 is a diagram showing the structure of a housing member that constitutes the sample preparation apparatus of the present embodiment; 本実施形態の試料作製装置を構成する固定部材の構造を示す図。FIG. 2 is a diagram showing the structure of a fixing member that constitutes the sample preparation apparatus of the present embodiment; 本実施形態における観察用試料の作製を説明する図。4A and 4B are diagrams for explaining preparation of an observation sample according to the present embodiment; FIG. 本実施形態において作製された試料のSEM画像およびその比較例。SEM images of samples produced in this embodiment and comparative examples thereof. 本実施形態の試料作製装置を構成する収容部材の第1の変形例を示す図。FIG. 4 is a diagram showing a first modification of the housing member that constitutes the sample preparation apparatus of the present embodiment; 本実施形態の試料作製装置を構成する収容部材の第2の変形例を示す図。The figure which shows the 2nd modification of the accommodating member which comprises the sample preparation apparatus of this embodiment. 本実施形態の試料作製装置を構成する収容部材の第3の変形例および固定部材の変形例を示す図。FIG. 10 is a diagram showing a third modification of the housing member and a modification of the fixing member, which constitute the sample preparation apparatus of the present embodiment; 本実施形態の試料作製装置を構成する収容部材の第3の変形例および固定部材の変形例を示す図。FIG. 10 is a diagram showing a third modification of the housing member and a modification of the fixing member, which constitute the sample preparation apparatus of the present embodiment; 従来技術における観察用試料の作製の概略を示す図。FIG. 11 is a diagram showing an outline of preparation of an observation sample in the conventional technology;

以下、本発明を、実施形態をもって説明するが、本発明は後述する実施形態に限定されるものではない。なお、以下に参照する各図においては、共通する要素について同じ符号を用い、適宜その説明を省略するものとする。 The present invention will be described below with reference to embodiments, but the present invention is not limited to the embodiments described later. In addition, in each figure referred to below, the same reference numerals are used for common elements, and description thereof will be omitted as appropriate.

また、以下に説明する実施形態では、微小生物を被観察物として、走査型電子顕微鏡(SEM)で観察するための試料を作製する場合を例示しているが、特に実施形態を限定するものではない。したがって、微小生物以外にも、食品、植物、細胞、ゲル状物などを被観察物としてもよく、さらにその応用として、化学、製薬などの分野において適用してもよい。また、観察装置についても、SEM以外の装置であってもよい。 In addition, in the embodiments described below, a case is exemplified in which a sample for observation with a scanning electron microscope (SEM) is prepared using micro-organisms as an object to be observed, but the embodiments are not particularly limited. do not have. Therefore, in addition to micro-organisms, foods, plants, cells, gel-like substances, etc. may be used as objects to be observed. Further, as an application thereof, the present invention may be applied in fields such as chemistry and pharmaceuticals. Also, the observation device may be a device other than the SEM.

図1は、本実施形態の試料作製装置10の構造を示す斜視図である。本実施形態の試料作製装置10は、収容部と固定部から構成され、図1に示すように、被観察物および水を収容する第1の収容部材11aおよび第2の収容部材11bと、第1の収容部材11aおよび第2の収容部材11bを固定する固定部材12およびネジ13とを具備する。なお、第1の収容部材11aおよび第2の収容部材11bを組み合わせることで、密閉された空間を形成することができる。また、図1では、固定のためのネジ13は、六角穴付きボルトが例として図示されているが、特に実施形態を限定するものではない。以下に説明する実施形態では、試料作製装置10に収容された被観察物および水をまとめて「内容物」として参照する場合がある。 FIG. 1 is a perspective view showing the structure of a sample preparation apparatus 10 of this embodiment. A sample preparation apparatus 10 of the present embodiment is composed of a storage section and a fixing section, and as shown in FIG. A fixing member 12 and a screw 13 are provided for fixing the first housing member 11a and the second housing member 11b. A closed space can be formed by combining the first housing member 11a and the second housing member 11b. In addition, in FIG. 1, the screw 13 for fixing is shown as an example of a hexagon socket head bolt, but the embodiment is not particularly limited. In the embodiments described below, the object to be observed and the water contained in the sample preparation device 10 may be collectively referred to as "contents."

図1に示した試料作製装置10を冷却し、収容した内容物を凍結させ、割断することで、氷晶の生成を抑制した顕微鏡観察用の試料を作製することができる。以下に、図1に示した本実施形態の試料作製装置10を構成する各部について、図2および図3を以て説明する。図2は、本実施形態の試料作製装置10を構成する収容部材11の構造を示す図であり、図3は、本実施形態の試料作製装置10を構成する固定部材12の構造を示す図である。 By cooling the sample preparation apparatus 10 shown in FIG. 1 and freezing and breaking the contained contents, it is possible to prepare a sample for microscopic observation in which formation of ice crystals is suppressed. Each part constituting the sample preparation apparatus 10 of the present embodiment shown in FIG. 1 will be described below with reference to FIGS. 2 and 3. FIG. FIG. 2 is a view showing the structure of a housing member 11 that constitutes the sample preparation apparatus 10 of this embodiment, and FIG. 3 is a view that shows the structure of a fixing member 12 that constitutes the sample preparation apparatus 10 of this embodiment. be.

まず、図2の収容部材11について説明する。図2(a)は、収容部材11の投影図を示している。図2(a)上段は、収容部材11の上面図を示し、図2(a)下段は、収容部材11を図2(a)上段のA-A’線で切断した断面図を示している。また、図2(b)左図は、収容部材11の斜視図を示し、図2(b)右図は、収容部材11を切断した断面の斜視図を示している。 First, the housing member 11 shown in FIG. 2 will be described. FIG. 2(a) shows a projection view of the housing member 11. FIG. The upper part of FIG. 2(a) shows a top view of the housing member 11, and the lower part of FIG. 2(a) shows a cross-sectional view of the housing member 11 taken along line AA' in the upper part of FIG. 2(a). . 2B shows a perspective view of the housing member 11, and FIG.

図2の各図に示すように、収容部材11は、被観察物などを収容する空洞部と、空洞部の1面が開口した開口部とを具備した構造である。また、収容部材11の空洞部には、図2に示すように、収容した被観察物の位置を固定しやすくするための窪みを設けてもよい。 As shown in FIGS. 2A and 2B, the housing member 11 has a structure including a hollow portion for housing an object to be observed and the like, and an opening in which one side of the hollow portion is open. Further, as shown in FIG. 2, the hollow portion of the housing member 11 may be provided with a recess for facilitating fixation of the position of the housed object to be observed.

本実施委形態の試料作製装置10は、2つの収容部材11a,11bの開口部を合わせて固定することで、各収容部材11a,11bの空洞部が連結し、被観察物および水を収容するための1つの閉じた空間(以下、単に「空間」として参照する)が形成される。この空間は、内容物で内部が充填され、密閉されているため、凍結時における内容物の膨張が収容部材11の内壁によって押さえ付けられ、内容物を加圧することができる。これによって、被観察物の氷晶の生成を抑制することができる。 In the sample preparation apparatus 10 of the present embodiment, the openings of the two housing members 11a and 11b are aligned and fixed so that the cavities of the housing members 11a and 11b are connected to accommodate the object to be observed and water. A closed space (hereinafter simply referred to as “space”) is formed for Since this space is filled with the content and sealed, the expansion of the content when frozen is suppressed by the inner wall of the housing member 11, and the content can be pressurized. As a result, it is possible to suppress the formation of ice crystals in the observed object.

なお、本実施形態の試料作製装置10を構成する第1の収容部材11aおよび第2の収容部材11bの形状は、必ずしも同一でなくてもよく、それぞれ異なる形状で構成されてもよい。 The shapes of the first housing member 11a and the second housing member 11b, which constitute the sample preparation apparatus 10 of the present embodiment, do not necessarily have to be the same, and they may have different shapes.

また、収容部材11の空洞部の大きさは、内容物を充分に凍結できる程度であれば特に限定されないが、一例として開口部の直径を8mm程度、深さを4mm程度とすることで、特許文献2や非特許文献1などの従来技術に比べて、格段に大きな被観察物であっても試料を作製することができる。 In addition, the size of the hollow portion of the containing member 11 is not particularly limited as long as the contents can be sufficiently frozen. Compared to the conventional techniques such as Document 2 and Non-Patent Document 1, a sample can be produced even for a much larger object to be observed.

次に、図3の固定部材12について説明する。図3(a)は、固定部材12の投影図を示している。また、図3(b)は、固定部材12の斜視図を示している。 Next, the fixing member 12 shown in FIG. 3 will be described. FIG. 3A shows a projection view of the fixing member 12. FIG. 3B shows a perspective view of the fixing member 12. FIG.

図3の各図に示すように、本実施形態の固定部材12は、枠型形状の部材であり、上部に貫通したネジ穴が設けられている。本実施形態の試料作製装置10は、固定部材12の枠内に、開口部を合わせた2つの収容部材11a,11bを収め、ネジ13で締めることで、各収容部材11a,11bを密閉して固定することができる(図1参照)。 As shown in FIGS. 3A and 3B, the fixing member 12 of the present embodiment is a frame-shaped member, and is provided with a through screw hole in the upper portion thereof. In the sample preparation apparatus 10 of the present embodiment, two housing members 11a and 11b are housed in the frame of the fixing member 12 with their openings aligned, and the housing members 11a and 11b are tightly closed by tightening them with screws 13. It can be fixed (see Figure 1).

なお、固定部材12の形状は、図3に示すような枠型形状に限定されない。すなわち、固定部材12は、開口部を合わせた2つの収容部材11a,11bを、ネジ13を占めることによって上方および下方から押さえ付けられる構造であればよく、例えば、「コの字」形状の固定部材12であってもよい。 In addition, the shape of the fixing member 12 is not limited to a frame shape as shown in FIG. That is, the fixing member 12 may have a structure in which the two holding members 11a and 11b with the openings aligned are pressed from above and below by occupying the screws 13. It may be member 12 .

また、説明する実施形態に係る試料作製装置10を構成する各部材は、構造がシンプルであるため、製造時における加工が容易であり、製造コストの面でも優れる。 In addition, since each member constituting the sample preparation apparatus 10 according to the embodiment to be described has a simple structure, it is easy to process during manufacturing, and is excellent in terms of manufacturing cost.

以上、図1~3に示した構造の試料作製装置10によって、氷晶の生成を抑制した試料を作製することができる。次に、本実施形態の試料作製装置10による凍結割断試料の作製について、図4を以て説明する。図4は、本実施形態における観察用試料の作製を説明する図である。本実施形態における試料の作製は、図4(a)~(c)の順序で行われる。 As described above, the sample preparation device 10 having the structure shown in FIGS. 1 to 3 can prepare a sample in which the formation of ice crystals is suppressed. Next, preparation of a freeze-fractured sample by the sample preparation apparatus 10 of this embodiment will be described with reference to FIG. FIG. 4 is a diagram for explaining preparation of an observation sample in this embodiment. The sample preparation in this embodiment is performed in the order of FIGS. 4(a) to 4(c).

まず、図4(a)に示すように、投入工程および固定工程を行う。すなわち、投入工程では、第1の収容部材11aおよび第2の収容部材11bに、被観察物および水を入れ、第1の収容部材11aおよび第2の収容部材11bの空洞部を内容物で充填する。なお、試料に不純物が混入するのを防ぐため、充填される水は、純水または超純水とすることが好ましい(説明する実施形態における「水」の用語は、純水および超純水をも含むものとする)。 First, as shown in FIG. 4A, a loading step and a fixing step are performed. That is, in the loading step, the object to be observed and water are put into the first containing member 11a and the second containing member 11b, and the hollow portions of the first containing member 11a and the second containing member 11b are filled with the contents. do. In order to prevent contamination of the sample with impurities, the water to be filled is preferably pure water or ultrapure water (the term "water" in the described embodiment means pure water and ultrapure water). shall also include).

投入工程の後、固定工程では、第1の収容部材11aの開口部と、第2の収容部材11bの開口部とを合わせて、固定部材12の内部に収め、ネジ13で締めつけることで、第1の収容部材11aおよび第2の収容部材11bを固定する。これによって、図1に示したような形態の試料作製装置10が構成される。 After the loading step, in the fixing step, the opening of the first housing member 11a and the opening of the second housing member 11b are aligned, housed inside the fixing member 12, and tightened with the screws 13 to secure the second housing member 11b. The first housing member 11a and the second housing member 11b are fixed. Thus, the sample preparation apparatus 10 having the form shown in FIG. 1 is constructed.

なお、好ましい実施形態では、図4(a)に示す投入工程および固定工程は、水中で行うこととしてもよい。これによって、試料作製装置10の密閉された空間に空気が入らず、空間内部が水で充填されるため、膨張による加圧を効果的に行うことができる。 In a preferred embodiment, the loading step and fixing step shown in FIG. 4(a) may be performed in water. As a result, air does not enter the sealed space of the sample preparation apparatus 10, and the space is filled with water, so that pressurization by expansion can be effectively performed.

また、密閉された空間の気密性を向上させるために、第1の収容部材11aおよび第2の収容部材11bを固定する際に、各収容部材11の間には、ガスケットを挿入してもよい。ガスケットの材料には、特に制限はないが、例えば感圧紙や銅などとすることができる。印加された圧力に応じて着色される感圧紙(例えば、富士フィルム社製「プレスケール(登録商標)」など)をガスケットに用いることで、固定工程において第1の収容部材11aおよび第2の収容部材11bが適当な圧力で固定されていることを視覚的に把握することができる。また、銅製のガスケットを挿入することで、後述する冷却工程における熱伝導を向上でき、効率的な冷却を行うことができる。特に銅製のガスケットを挿入した場合には、感圧紙を用いた場合に比べて、氷晶の生成がより効果的に抑制されていることが確認された。 Further, in order to improve the airtightness of the sealed space, a gasket may be inserted between each housing member 11 when fixing the first housing member 11a and the second housing member 11b. . The gasket material is not particularly limited, but pressure-sensitive paper, copper, or the like can be used, for example. By using pressure-sensitive paper that is colored according to the applied pressure (for example, "Prescale (registered trademark)" manufactured by Fuji Film Co., Ltd.) as a gasket, the first housing member 11a and the second housing member 11a are separated from each other in the fixing step. It can be visually recognized that the member 11b is fixed with an appropriate pressure. Also, by inserting a copper gasket, it is possible to improve heat conduction in the cooling process, which will be described later, and to perform efficient cooling. In particular, it was confirmed that when a copper gasket was inserted, the formation of ice crystals was suppressed more effectively than when pressure-sensitive paper was used.

投入工程および固定工程のあと、図4(b)に示すように冷却工程を行い、試料作製装置10の内容物を凍結させる。図4(b)は、試料作製装置10の第1の収容部材11aおよび第2の収容部材11bを拡大した断面図である。図4(b)に示すように、試料作製装置10の密閉された空間は、内容物で充填され、内部が満たされている。したがって、試料作製装置10が冷却されて、内容物が凍結されると、凍結に伴う内容物の膨張によって、内部が加圧される。これによって、氷晶の生成を抑制することができる。 After the loading process and the fixing process, the cooling process is performed as shown in FIG. FIG. 4(b) is an enlarged cross-sectional view of the first housing member 11a and the second housing member 11b of the sample preparation apparatus 10. FIG. As shown in FIG. 4(b), the closed space of the sample preparation device 10 is filled with contents to fill the inside. Therefore, when the sample preparation device 10 is cooled and the contents are frozen, the inside is pressurized due to the expansion of the contents due to freezing. This can suppress the formation of ice crystals.

なお、冷却工程における試料作製装置10を冷却する方法は、特に限定されず、種々の方法を採用することができる。冷却方法の一例として、試料作製装置10を液体窒素に浸漬する方法が挙げられるが、液体窒素以外の冷却材料を用いてもよい。 A method for cooling the sample preparation apparatus 10 in the cooling step is not particularly limited, and various methods can be adopted. An example of the cooling method is a method of immersing the sample preparation device 10 in liquid nitrogen, but a cooling material other than liquid nitrogen may be used.

冷却工程によって内容物を凍結させたあと、図4(c)に示す割断工程を行う。割断工程では、試料作製装置10の固定を外し、第1の収容部材11aおよび第2の収容部材11bを分離する。また、凍結によって膨張した氷は、収容部の内壁に押さえられているため、割断工程では、第1の収容部材11aおよび第2の収容部材11bを把持し、連結部分を折るようにして分離させることで、凍結した被観察物が割断され、割断面を露出させることができる。なお、各収容部材11を分離しやするするために、連結部分に刃を入れ、氷に切れ目を入れてから割断してもよい。割断工程によって露出した割断面は、顕微鏡観察における観察面となる。その後、被測定物を真空乾燥させ、オスミウムコーティングを行うことで、SEM観察用試料として完成し、SEMによる観察を行うことができる。 After the contents are frozen by the cooling process, the cutting process shown in FIG. 4(c) is performed. In the cutting step, the sample preparation device 10 is released and the first housing member 11a and the second housing member 11b are separated. In addition, since the ice that has expanded due to freezing is held down by the inner wall of the storage portion, in the cutting step, the first storage member 11a and the second storage member 11b are grasped and separated by folding the connecting portions. As a result, the frozen object to be observed is cleaved, and the cleaved surface can be exposed. In addition, in order to facilitate the separation of the storage members 11, a blade may be inserted into the connecting portion to cut the ice before cutting. The cut surface exposed by the cutting step serves as an observation surface in microscopic observation. Thereafter, the object to be measured is vacuum-dried and coated with osmium to complete a sample for SEM observation, which can be observed by SEM.

図4において説明した各工程によって、水分を含む被観察物であっても、氷晶の生成によるダメージを抑制して観察用試料を作製することができる。また、図10に示した従来技術などでは、1mm以下(0.06ミリリットル程度)の小さな被観察物の試料しか作製できなかったが、本実施形態の試料作製では、0.4ミリリットル以上の比較的大きな被観察物であっても観察用試料を作製することができる。さらに、本実施形態における試料作製の冷却工程では、図10に示した従来技術などよりも遅い冷却速度であっても、氷晶の生成を抑制することができる。 Through the steps described with reference to FIGS. 4A and 4B, it is possible to prepare an observation sample while suppressing damage due to formation of ice crystals even for an object to be observed containing moisture. In the prior art shown in FIG. 10, only a small sample of 1 mm or less (approximately 0.06 ml) can be produced. Observation specimens can be prepared even for large objects to be observed. Furthermore, in the cooling step for sample preparation in the present embodiment, the formation of ice crystals can be suppressed even if the cooling rate is lower than that of the prior art shown in FIG.

図5は、本実施形態において作製された試料のSEM画像およびその比較例である。図5における試料は、2%寒天ゲルを被観察物として凍結し割断したものである。図5(A)および(a-1)~(a-3)は、2%寒天ゲルを本実施形態の方法で凍結し、割断して作製された試料を、SEMで観察した画像である。また、図5(B)および(b-1)~(b-3)は、本実施形態との比較例であり、2%寒天ゲルを液体窒素に浸漬させ、SEMで観察した画像である。 FIG. 5 is an SEM image of a sample produced in this embodiment and its comparative example. The sample in FIG. 5 is obtained by freezing and breaking a 2% agar gel as an object to be observed. FIGS. 5(A) and (a-1) to (a-3) are SEM images of a sample prepared by freezing and breaking a 2% agar gel by the method of the present embodiment. FIGS. 5B and 5B and 5B-1 to 5B-3 are comparative examples with this embodiment, and are images of 2% agar gel immersed in liquid nitrogen and observed with SEM.

まず、図5(A)および(a-1)~(a-3)について説明する。図5(A)は、本実施形態の方法によって作製された試料全体のSEM画像である。また、図5(a-1)~(a-3)は、それぞれ図5(A)中の1~3の位置を拡大したSEM画像である。図5(a-1)は、試料の外側近傍のSEM画像であり、わずかに寒天の網目構造がダメージを受けていることが観察された。図5(a-2)は、試料表面から1mm程度内側の部分のSEM画像であり、寒天特有の良好な網目構造が観察された。また、図5(a-3)は、試料の中央付近のSEM画像であり、寒天特有の良好な網目構造が観察された。すなわち、本実施形態の方法によって作製された試料のいずれの部位においても、寒天に特有の網目構造が観察され、特に、図5(a-2)および(a-3)では、良好な網目構造が観察されたことから、本実施形態の方法によって、凍結時における氷晶の生成が抑制されていることが確認された。 First, FIGS. 5(A) and (a-1) to (a-3) will be described. FIG. 5A is an SEM image of the entire sample produced by the method of this embodiment. 5(a-1) to (a-3) are SEM images in which positions 1 to 3 in FIG. 5(A) are enlarged, respectively. FIG. 5(a-1) is an SEM image near the outside of the sample, and it was observed that the network structure of the agar was slightly damaged. FIG. 5(a-2) is an SEM image of a portion about 1 mm inside from the surface of the sample, and a good network structure peculiar to agar was observed. Further, FIG. 5(a-3) is an SEM image of the vicinity of the center of the sample, in which a good network structure peculiar to agar was observed. That is, in any part of the sample prepared by the method of the present embodiment, a network structure peculiar to agar was observed, and in particular, in FIGS. was observed, it was confirmed that the method of the present embodiment suppresses the formation of ice crystals during freezing.

次に、図5(B)および(b-1)~(b-3)について説明する。図5(B)は、2%寒天ゲルを液体窒素に浸漬させることで作製された試料のSEM画像である。また、図5(b-1)~(b-3)は、それぞれ図5(B)中の1~3の位置を拡大したSEM画像であり、図5(b-1)は、試料の外側近傍を、図5(b-2)は、試料表面から1mm程度内側の部分を、図5(a-3)は、試料の中央付近を、それぞれ示している。図5(b-1)、(b-2)に示すように、2%寒天ゲルを液体窒素に浸漬させて作製した試料の外周に近い部位は、氷晶の生成による被観察物へのダメージが確認された。また、図5(b-3)に示すように、試料の中央付近では、寒天の網目構造がみられるが、網目が比較的大きいことから、氷晶の生成が認められ、被観察物へのダメージが確認された。 Next, FIGS. 5B and 5B-1 to 5B-3 will be described. FIG. 5(B) is an SEM image of a sample prepared by immersing a 2% agar gel in liquid nitrogen. 5(b-1) to (b-3) are SEM images in which positions 1 to 3 in FIG. 5(B) are enlarged, respectively, and FIG. 5(b-1) is the outside of the sample. FIG. 5(b-2) shows the part about 1 mm inside from the sample surface, and FIG. 5(a-3) shows the vicinity of the center of the sample. As shown in FIGS. 5(b-1) and 5(b-2), the portion near the outer periphery of the sample prepared by immersing 2% agar gel in liquid nitrogen is damaged by the generation of ice crystals. was confirmed. In addition, as shown in FIG. 5(b-3), a network structure of agar can be seen near the center of the sample. Damage confirmed.

図5に示したように、本実施形態の方法で作製した試料は、寒天特有の網目構造が確認され、氷晶の生成が抑制されていることを確認した。したがって、本実施形態の方法によって、水分の含有量が多い被観察物であっても、氷晶の生成を抑制して試料を作製できたことが確認できた。 As shown in FIG. 5, the sample prepared by the method of the present embodiment was confirmed to have a network structure unique to agar, and it was confirmed that the formation of ice crystals was suppressed. Therefore, it was confirmed that, by the method of the present embodiment, a sample could be produced by suppressing the formation of ice crystals even with an object to be observed having a high water content.

ここまでに説明した実施形態では、図2に例示した形状の収容部材11で以て説明した。しかしながら、収容部材11の形状は、図2に示したものに限定されず、例えば、以下に示す各変形例のような形状であってもよい。 In the embodiments described so far, the housing member 11 having the shape illustrated in FIG. 2 has been described. However, the shape of the housing member 11 is not limited to that shown in FIG. 2, and may be, for example, a shape such as each modification shown below.

まず、第1の変形例について説明する。図6は、本実施形態の試料作製装置10を構成する収容部材11の第1の変形例を示す図である。図6(a)は、収容部材11の第1の変形例の上面投影図および側面断面の投影図であり、図6(b)は、斜視図および断面斜視図である。図6に示すように、第1の変形例における収容部材11は、空洞部が開口部に向かって狭くなる形状である。このような形状とすることで、第1の収容部材11aの開口部と、第2の収容部材11bの開口部とが連結する面積が小さくなることから、各収容部材11を分離しやすくでき、割断工程を容易に行うことができる。 First, a first modified example will be described. FIG. 6 is a diagram showing a first modification of the housing member 11 that constitutes the sample preparation apparatus 10 of this embodiment. FIG. 6(a) is a top projection view and a side cross-sectional projection view of a first modified example of the housing member 11, and FIG. 6(b) is a perspective view and a cross-sectional perspective view. As shown in FIG. 6, the housing member 11 in the first modified example has a shape in which the cavity narrows toward the opening. With such a shape, the area where the opening of the first housing member 11a and the opening of the second housing member 11b are connected becomes small, so that the housing members 11 can be easily separated. The cutting process can be easily performed.

次に、第2の変形例について説明する。図7は、本実施形態の試料作製装置10を構成する収容部材11の第2の変形例を示す図である。図7(a)は、収容部材11の第2の変形例の上面投影図および側面断面の投影図であり、図7(b)は、第2の変形例に係る収容部材11によって構成される試料作製装置10の斜視図である。図7に示す第2の変形例に係る収容部材11は、本実施形態の収容部と固定部とを一体として構成された形状である。 Next, a second modified example will be described. FIG. 7 is a diagram showing a second modification of the housing member 11 that constitutes the sample preparation apparatus 10 of this embodiment. FIG. 7(a) is a top projection view and a side cross-sectional projection view of a second modification of the housing member 11, and FIG. 7(b) is configured by the housing member 11 according to the second modification. 1 is a perspective view of a sample preparation device 10; FIG. A housing member 11 according to a second modification shown in FIG. 7 has a shape in which the housing portion and the fixing portion of the present embodiment are integrated.

図7(a)に示すように、第2の変形例の収容部材11は、図2などで説明した空洞部および開口部を備え、さらに、開口部の開口面にフランジ部を具備する。フランジ部には、同一円周上に等配された穴が設けられている。フランジ部は、固定部材12に相当する機能を有し、固定工程においてネジ留めされることで、第1の収容部材11aおよび第2の収容部材11bを固定することができる。なお、フランジ部の穴の位置や数は、図7に示したものに限定されず、任意とすることができる。また、フランジ部の穴は、タッピング処理されたネジ穴であってもよい。 As shown in FIG. 7(a), the housing member 11 of the second modification includes the cavity and the opening described in FIG. 2 and the like, and further includes a flange on the opening surface of the opening. The flange portion is provided with holes evenly distributed on the same circumference. The flange portion has a function corresponding to the fixing member 12, and can fix the first housing member 11a and the second housing member 11b by being screwed in the fixing process. The positions and number of holes in the flange portion are not limited to those shown in FIG. 7, and may be arbitrary. Also, the holes in the flange portion may be tapped screw holes.

第2の変形例に係る収容部材11は、図7(b)左図のように組み合わせることで、試料作製装置10を構成する。すなわち、フランジ部付きの収容部材11を、第1の収容部材11aおよび第2の収容部材11bとして、開口部およびフランジ部の穴を合わせ、ネジ13およびナット13aで固定する。これによって、図7(b)右図のような形態の試料作製装置10とすることができる。第2の変形例に係る収容部材11を用いることで、固定部材12が不要な試料作製装置10とすることができる。 The storage member 11 according to the second modification constitutes the sample preparation device 10 by combining them as shown in the left diagram of FIG. 7(b). That is, the housing member 11 with flanges is used as the first housing member 11a and the second housing member 11b, and the holes of the opening and the flange are aligned and fixed with screws 13 and nuts 13a. As a result, the sample preparation apparatus 10 can be configured as shown in the right diagram of FIG. 7(b). By using the housing member 11 according to the second modification, the sample preparation apparatus 10 can be made without the fixing member 12 .

次に第3の変形例について説明する。図8および図9は、本実施形態の試料作製装置10を構成する収容部材11の第3の変形例および固定部材12の変形例を示す図である。 Next, a third modified example will be described. 8 and 9 are diagrams showing a third modified example of the housing member 11 and a modified example of the fixing member 12 that constitute the sample preparation apparatus 10 of this embodiment.

収容部材11の第3の変形例は、図8(a)および(b)に示すように、台1の収容部材11aと第2の収容部材11bとで異なる形状である。すなわち、第1の収容部材11aは、図2に示した収容部材11と同様の形状である。なお、第1の収容部材11aには、図8(a)に示すように、後述するようにピン14を挿入するための穴を設けることが好ましい。また、第2の収容部材11bは、図8(b)に示すように、図2に示した収容部材11にテーパ状の穴が設けられており、開口部からテーパ部まで貫通した形状である。なお、固定部材12は、図8(c)に示すように、図3に示したものと同様の形状であるが、図8(a)に示した収容部材11aのピン挿入穴に対応する穴が設けられていてもよい。 In a third modification of the housing member 11, as shown in FIGS. 8A and 8B, the housing member 11a and the second housing member 11b of the table 1 have different shapes. That is, the first housing member 11a has the same shape as the housing member 11 shown in FIG. In addition, as shown in FIG. 8A, it is preferable to provide a hole for inserting a pin 14 as described later in the first housing member 11a. Further, as shown in FIG. 8B, the second housing member 11b is provided with a tapered hole in the housing member 11 shown in FIG. . As shown in FIG. 8C, the fixing member 12 has the same shape as that shown in FIG. may be provided.

上述した各収容部材11および固定部材12を用いた試料作製装置10は、図9(a)に示すように構成される。図9(a)は、図8に示した各部材を用いた試料作製装置10における、投入工程・固定工程を示している。ここで、収容部材11および固定部材12を固定するためのネジは、図9(a)に示すように、先端にテーパ形状を有するネジ13’(以下、「テーパ付きネジ13’」として参照する)を用いる。テーパ付きネジ13’は、先端部のテーパ形状が第2の収容部材11bのテーパ部に対応する形状であり、固定工程において、テーパ付きネジ13’のテーパ部と、第2の収容部材11bのテーパ部分とが密着する。 A sample preparation apparatus 10 using the above-described housing member 11 and fixing member 12 is configured as shown in FIG. 9(a). FIG. 9(a) shows a loading step and a fixing step in the sample preparation apparatus 10 using each member shown in FIG. Here, as shown in FIG. 9A, the screw for fixing the housing member 11 and the fixing member 12 is a screw 13' having a tapered tip (hereinafter referred to as a "tapered screw 13'"). ) is used. The tapered screw 13' has a tapered shape at the tip corresponding to the tapered portion of the second housing member 11b. The tapered portion is in close contact.

図9(b)は、試料作製装置10の断面図である。なお、図9(b)では、被観察物や水などが省略して図示されている点に留意されたい。図9(b)に示すように、テーパ付きネジ13’を用いることによって、収容部材11aおよび11bを固定するとともに、空間を密閉することができ、冷却工程における加圧を可能とする。また、第1の収容部材11aと、固定部材12とにピン14を挿入することで、各部材のズレを防止することができる。 FIG. 9B is a cross-sectional view of the sample preparation device 10. FIG. Note that the object to be observed, water, and the like are omitted in FIG. 9B. As shown in FIG. 9(b), by using the tapered screw 13', it is possible to fix the containing members 11a and 11b, to seal the space, and to pressurize in the cooling process. Further, by inserting the pin 14 into the first housing member 11a and the fixing member 12, it is possible to prevent the respective members from being displaced.

図8および図9に示した形態の試料作製装置10を用いることによって、各工程の作業性を向上することができる。 By using the sample preparation apparatus 10 having the configuration shown in FIGS. 8 and 9, the workability of each step can be improved.

以上に説明した本発明の実施形態によれば、氷晶の生成を抑制する試料作製方法、凍結加圧装置および観察方法を提供することができる。また、本実施形態は、簡易な構成で以て氷晶の生成を抑制できることから、コスト低減にも寄与し得る。さらに、従来技術よりも格段に大きな試料を作製することができる。 According to the embodiments of the present invention described above, it is possible to provide a sample preparation method, a freezing pressurization device, and an observation method that suppress the formation of ice crystals. In addition, since the present embodiment can suppress the formation of ice crystals with a simple structure, it can contribute to cost reduction. Furthermore, significantly larger samples can be made than in the prior art.

以上、本発明について実施形態をもって説明してきたが、本発明は上述した実施形態に限定されるものではなく、当業者が推考しうる実施態様の範囲内において、本発明の作用・効果を奏する限り、本発明の範囲に含まれるものである。また、説明した実施形態に係る試料作製装置は、観察用試料を作製するための用途に供されるものに限定されず、水の凍結によって内容物を加圧するため装置などであってもよい。 As described above, the present invention has been described with embodiments, but the present invention is not limited to the above-described embodiments, and within the scope of embodiments that can be conceived by those skilled in the art, as long as the actions and effects of the present invention are exhibited. , are within the scope of the present invention. Further, the sample preparation device according to the described embodiments is not limited to one used for preparing observation samples, and may be a device for pressurizing contents by freezing water.

10…試料作製装置、
11…収容部材、
12…固定部材、
13…ネジ、
13’…テーパ付きネジ、
13a…ナット、
14…ピン、
50…平板型試料作製装置、
51…平板型収容部材 10 ... sample preparation device,
11 ... accommodation member,
12... Fixing member,
13... screw,
13'...tapered screw,
13a ... nut,
14... pin,
50... Plate type sample preparation device,
51... Flat plate type housing member

特開2013-253957号公報JP 2013-253957 A 特開2014-25732号公報JP 2014-25732 A

太田裕彦 et al. (2011):冷却水を使用した新しいSEM試料作製用凍結乾燥法.医学生物学電子顕微鏡技術学会誌,25(1):9-13.Hirohiko Ohta et al. (2011): New freeze-drying method for SEM sample preparation using cooling water. Journal of the Society of Medical and Biological Electron Microscopy, 25(1):9-13.

Claims (11)

空洞部と、前記空洞部の1つの面が開口した開口部とを有する第1の部材および第2の部材からなる試料作製装置の内部の空間に、被観察物および水を入れて、前記空間に充填する工程と、
前記第1の部材の開口部と、前記第2の部材の開口部とを合わせて固定する工程と、
前記試料作製装置を冷却する工程と、
前記第1の部材および前記第2の部材を分離して、前記冷却する工程によって凍結した前記被観察物を割断する工程と
を含む、試料作製方法。 An object to be observed and water are put into a space inside a sample preparation device comprising a first member and a second member having a hollow portion and an opening with one side of the hollow portion open, and the space is filled with water. filling into
aligning and fixing the opening of the first member and the opening of the second member;
a step of cooling the sample preparation device;
and a step of separating the first member and the second member, and cutting the frozen observation object by the cooling step. 前記充填する工程は、水中で行われることを特徴とする、請求項1に記載の試料作製方法。 2. The sample preparation method according to claim 1, wherein said filling step is performed in water. 前記割断する工程は、前記第1の部材と前記第2の部材とが連結した部分を折ることで、前記第1の部材および前記第2の部材を分離することを特徴とする、請求項1または2に記載の試料作製方法。 2. The step of breaking the first member and the second member by folding a portion where the first member and the second member are connected to separate the first member and the second member. 3. or the sample preparation method according to 2. 空洞部と、前記空洞部の1つの面が開口した開口部とを有する第1の収容部および第2の収容部と、
前記第1の収容部と前記第2の収容部とを固定する固定部と
を具備し、
前記第1の収容部の開口部と、前記第2の収容部の開口部とを合わせて、前記固定部によって固定して形成される空間を有する、
凍結加圧装置。 a first accommodating portion and a second accommodating portion each having a hollow portion and an opening in which one surface of the hollow portion is open;
a fixing part that fixes the first accommodation part and the second accommodation part,
Having a space formed by combining the opening of the first accommodating portion and the opening of the second accommodating portion and fixing it by the fixing portion,
Freezing pressure device. 前記空洞部は、前記開口部に向かって狭くなることを特徴とする、請求項4に記載の凍結加圧装置。 5. The freeze pressurization device of claim 4, wherein said cavity narrows towards said opening. 前記第1の収容部および前記第2の収容部は、それぞれが前記固定部と一体として構成されることを特徴とする、請求項4または5に記載の凍結加圧装置。 6. The freezing and pressurizing device according to claim 4, wherein the first accommodating portion and the second accommodating portion are each configured integrally with the fixing portion. 前記第2の収容部は、開口部の反対側に開いたテーパ部を有し、前記テーパ部に対応する形状を具備するネジによって、前記第1の収容部と前記第2の収容部とを固定することを特徴とする、請求項4または5に記載の凍結加圧装置。 The second accommodating portion has a tapered portion that opens on the opposite side of the opening, and a screw having a shape corresponding to the tapered portion connects the first accommodating portion and the second accommodating portion. 6. A freezing pressurization device according to claim 4 or 5, characterized in that it is fixed. 前記第1の収容部の開口部と、前記第2の収容部の開口部との間にガスケットを挿入して、前記固定部によって固定することを特徴とする、請求項4~7のいずれか1項に記載の凍結加圧装置。 Any one of claims 4 to 7, characterized in that a gasket is inserted between the opening of the first accommodating portion and the opening of the second accommodating portion and fixed by the fixing portion. 2. The freeze pressurization device according to item 1. 前記ガスケットの材料が銅であることを特徴とする、請求項8に記載の凍結加圧装置。 9. The freezing pressurization device according to claim 8, wherein the material of said gasket is copper. 前記ガスケットは、印加された圧力に応じて着色されることを特徴とする、請求項8に記載の凍結加圧装置。 9. The freeze pressurization device of claim 8, wherein the gasket is colored according to the pressure applied. 空洞部と、前記空洞部の1つの面が開口した開口部とを有する第1の部材および第2の部材からなる試料作製装置の内部の空間に、被観察物および水を入れて、前記空間に充填する工程と、
前記第1の部材の開口部と、前記第2の部材の開口部とを合わせて固定する工程と、
前記試料作製装置を冷却する工程と、
前記第1の部材および前記第2の部材を分離して、前記冷却する工程によって凍結した前記被観察物を割断する工程と、
前記割断する工程によって割断された前記被観察物の割断面を観察する工程と
を含む、観察方法。

An object to be observed and water are put into a space inside a sample preparation device comprising a first member and a second member having a hollow portion and an opening with one side of the hollow portion open, and the space is filled with water. filling into
aligning and fixing the opening of the first member and the opening of the second member;
a step of cooling the sample preparation device;
a step of separating the first member and the second member and cutting the frozen observation object by the cooling step;
and a step of observing a fractured surface of the object to be observed that has been fractured by the fractured step.
JP2019211101A 2019-11-22 2019-11-22 Sample preparation method, freeze pressurization device, and observation method Pending JP2023022846A (en)

Priority Applications (3)

Application Number Priority Date Filing Date Title
JP2019211101A JP2023022846A (en) 2019-11-22 2019-11-22 Sample preparation method, freeze pressurization device, and observation method
JP2021558232A JPWO2021100396A1 (en) 2019-11-22 2020-10-21
PCT/JP2020/039620 WO2021100396A1 (en) 2019-11-22 2020-10-21 Sample preparation method, freezing and pressing device, and observation method

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
JP2019211101A JP2023022846A (en) 2019-11-22 2019-11-22 Sample preparation method, freeze pressurization device, and observation method

Publications (1)

Publication Number Publication Date
JP2023022846A true JP2023022846A (en) 2023-02-16

Family

ID=75981606

Family Applications (2)

Application Number Title Priority Date Filing Date
JP2019211101A Pending JP2023022846A (en) 2019-11-22 2019-11-22 Sample preparation method, freeze pressurization device, and observation method
JP2021558232A Pending JPWO2021100396A1 (en) 2019-11-22 2020-10-21

Family Applications After (1)

Application Number Title Priority Date Filing Date
JP2021558232A Pending JPWO2021100396A1 (en) 2019-11-22 2020-10-21

Country Status (2)

Country Link
JP (2) JP2023022846A (en)
WO (1) WO2021100396A1 (en)

Family Cites Families (7)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPH01142436A (en) * 1987-11-30 1989-06-05 Ushio Inc Apparatus for splitting frozen solid specimen
JPH0829303A (en) * 1994-07-20 1996-02-02 Osaka Oxygen Ind Ltd Metal specimen take-out apparatus
JP3781723B2 (en) * 2002-12-20 2006-05-31 日本電子株式会社 Sample holder for freezing breakage of high-pressure freezing apparatus and high-pressure freezing apparatus
JP3839407B2 (en) * 2003-01-07 2006-11-01 株式会社日立ハイテクノロジーズ Broken sample preparation method, sample observation method, and broken sample preparation apparatus
US7197884B2 (en) * 2004-03-01 2007-04-03 Christopher Jones Assembly and method for cryo-preservation of specimens in a cryogen-free environment
JP2009036694A (en) * 2007-08-03 2009-02-19 Tokyo Medical & Dental Univ Method for analyzing biological substance in cell maintaining spatial distribution
CN101959601A (en) * 2008-01-07 2011-01-26 哈维德夫医院 A storage vessel and a break tool for dividing such vessel

Also Published As

Publication number Publication date
WO2021100396A1 (en) 2021-05-27
JPWO2021100396A1 (en) 2021-05-27

Similar Documents

Publication Publication Date Title
Boyde et al. Preparation of animal tissues for surface‐scanning electron microscopy
US8151593B2 (en) Embedding method and apparatus for the preparation of frozen section tissue
Zhang et al. Intrinsic wettability in pristine graphene
Choi et al. Complete determination of the crystallographic orientation of ReX 2 (X= S, Se) by polarized Raman spectroscopy
Leunissen et al. Self‐pressurized rapid freezing (SPRF): a novel cryofixation method for specimen preparation in electron microscopy
JP6143487B2 (en) Method for making a vitrified sample for an electron microscope
JP6251708B2 (en) Operation container for cryomicroscopy
Walther et al. Double‐layer coating for high‐resolution low‐temperature scanning electron microscopy
JP2007165271A (en) Hermetically sealed observation environment forming device for electron microscope
WO2014002700A1 (en) Cryogenic specimen holder and cooling source container
JP2013156218A (en) Capillary for minute sample
JP6317900B2 (en) Capillary capillaries and caps for use in high pressure refrigerators
JP6294017B2 (en) Preparation of electron microscope samples from high-pressure refrigeration materials
JP2023022846A (en) Sample preparation method, freeze pressurization device, and observation method
Kleinerman et al. Cryogenic‐temperature electron microscopy direct imaging of carbon nanotubes and graphene solutions in superacids
Nijsse et al. Cryo‐planing for cryo‐scanning electron microscopy
Giese et al. The evolution of polycyclic aromatic hydrocarbons under simulated inner asteroid conditions
Sauer et al. Freeze-trapping isomorphous xenon derivatives of protein crystals
Edelmann A simple freeze‐drying technique for preparing biological tissue without chemical fixation for electron microscopy
JP2014025732A (en) Device and method for preparing frozen sample
Zierold Preparation of cryosections for biological microanalysis
US20070048792A1 (en) Preparing biological samples for analysis
TW201504439A (en) Cryopreservation storage device for blood bag and using method thereof
Payre et al. A new HPF specimen carrier adapter for the use of high‐pressure freezing with cryoscanning electron microscope: two applications: stearic acid organization in a hydroxypropyl methylcellulose matrix and mice myocardium
CN107991330B (en) Device and method for preparing liquid nitrogen mud frozen sample

Legal Events

Date Code Title Description
A80 Written request to apply exceptions to lack of novelty of invention

Free format text: JAPANESE INTERMEDIATE CODE: A80

Effective date: 20191205

RD03 Notification of appointment of power of attorney

Free format text: JAPANESE INTERMEDIATE CODE: A7423

Effective date: 20220829

A521 Request for written amendment filed

Free format text: JAPANESE INTERMEDIATE CODE: A821

Effective date: 20220829

A621 Written request for application examination

Free format text: JAPANESE INTERMEDIATE CODE: A621

Effective date: 20221108

A711 Notification of change in applicant

Free format text: JAPANESE INTERMEDIATE CODE: A711

Effective date: 20221115

A521 Request for written amendment filed

Free format text: JAPANESE INTERMEDIATE CODE: A821

Effective date: 20221115

A131 Notification of reasons for refusal

Free format text: JAPANESE INTERMEDIATE CODE: A131

Effective date: 20231121

A02 Decision of refusal

Free format text: JAPANESE INTERMEDIATE CODE: A02

Effective date: 20240514