JPH0933531A - Method for deciding presence of lung cancer cell and examination medicine for diagnosing lung cancer - Google Patents
Method for deciding presence of lung cancer cell and examination medicine for diagnosing lung cancerInfo
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- JPH0933531A JPH0933531A JP20665995A JP20665995A JPH0933531A JP H0933531 A JPH0933531 A JP H0933531A JP 20665995 A JP20665995 A JP 20665995A JP 20665995 A JP20665995 A JP 20665995A JP H0933531 A JPH0933531 A JP H0933531A
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- vpf
- lung cancer
- serum
- immunoassay
- diagnosing
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Abstract
Description
【0001】[0001]
【発明の属する技術分野】本発明は、血清中に存在する
血管透過性因子(vascular permeability factor)または
血管内皮細胞増殖因子(vascular endothelial growth f
actor)と呼称されている因子(以下VPFと略す)の存在
量を測定し、それに基づいて該血清提供者が肺癌細胞を
有するか否かを判定する方法に関するものであり、医者
が肺癌を診断する際に有用となる情報を提供する方法で
あり、また肺癌の診断に有用な肺癌診断用検査薬に関す
るものであり、医薬業界において利用されるものであ
る。TECHNICAL FIELD The present invention relates to a vascular permeability factor or a vascular endothelial growth factor present in serum.
The present invention relates to a method for determining whether or not the serum donor has lung cancer cells based on the measurement of the abundance of a factor called an actor) (hereinafter abbreviated as VPF), in which a doctor diagnoses lung cancer. The present invention relates to a method for providing useful information when carrying out the method, a test agent for diagnosing lung cancer useful for diagnosing lung cancer, and is used in the pharmaceutical industry.
【0002】[0002]
【従来の技術】現在、肺癌の早期診断としては一般的に
はX線検査が用いられている。一方、血清腫瘍マーカー
についても検討が進められ、CEA(carcinoembryonic
antigen)、SCC(squamous cell carcinoma-related a
ntigen)、NSE(neurospecific enolase) 、SLX(si
alyl LeX-i antigen)などが報告されているが、それら
の臨床病期I期の陽性率は高いものでも約30%である
(有吉 寛、桑原正喜:腫瘍マーカーの臨床への応用、
肺癌、病理と臨床、8、臨時増刊号 289-299、1990)。
従って、これらのマーカーは早期診断のために適当なも
のであるとは言えないものである。この原因としては、
これらの腫瘍マーカーの多くは、組織型により陽性率が
異なっている、すなわち、SCCは扁平上皮癌、SLX
は腺癌、NSEは小細胞癌において高い陽性率を示す
が、その他の組織型では陽性率は低いという様に、これ
らの腫瘍マーカーの産生は組織型が異なる細胞におい
て、発現量が異なっているということが考えられてい
る。一方、血管新生すなわち毛細血管内皮細胞の増殖、
移動および組織への浸潤という現象は胎児の生長、創傷
治癒、癌細胞の増殖などの生理的または病理的現象にお
いて重要な役割を果たしていることが知られており[(Fo
lkman,J.,Cancer Res.46:467(1986)]、血管新生を誘導
する因子としては、直接的に血管内皮細胞に作用する物
質として塩基性線維芽細胞増殖因子(basic fibroblast
growth factor,bFGF)、酸性線維芽細胞増殖因子(acidic
fibroblast growth factor,aFGF)、血管内皮細胞増殖
因子/血管透過性因子(vascular endothelial growth f
actor/vascular permeability factor,VPF)、血小板
由来内皮細胞増殖因子(platelet-derived endothelial
cell growth factor,PD-ECGF)などが、また間接的に血
管内皮細胞に作用する物質としてtransforming growth
factor-α(TGF-α)、transforming growth factor-β(T
GF-β)、angiogenin、tumor necrosis factor-α(TNF-
α)などが見つけられている[Folkman,J. & Shing,Y.,J.
Biol.Chem.,267:10931(1992)]。2. Description of the Related Art At present, X-ray examination is generally used as an early diagnosis of lung cancer. On the other hand, studies on serum tumor markers have been conducted, and CEA (carcinoembryonic
antigen), SCC (squamous cell carcinoma-related a
ntigen), NSE (neurospecific enolase), SLX (si
Alyl LeX-i antigens) have been reported, but their positive rate in clinical stage I is about 30%, even though they are high (Hiroshi Ariyoshi, Masayoshi Kuwahara: clinical application of tumor markers,
Lung cancer, pathology and clinic, 8, Extra edition 289-299, 1990).
Therefore, these markers are not suitable for early diagnosis. This can be caused by
Many of these tumor markers have different positive rates depending on the tissue type, that is, SCC is squamous cell carcinoma, SLX
Shows high positive rate in adenocarcinoma and NSE in small cell carcinoma, but low positive rate in other tissue types. Therefore, the expression levels of these tumor markers are different in cells of different tissue types. It is considered that. On the other hand, angiogenesis, the proliferation of capillary endothelial cells,
It is known that the phenomena of migration and tissue infiltration play important roles in physiological and pathological phenomena such as fetal growth, wound healing, and cancer cell proliferation [(Fo
lkman, J., Cancer Res. 46: 467 (1986)], as a factor that induces angiogenesis, basic fibroblast growth factor (basic fibroblast growth factor) is a substance that directly acts on vascular endothelial cells.
growth factor (bFGF), acidic fibroblast growth factor (acidic
fibroblast growth factor, aFGF), vascular endothelial growth factor
actor / vascular permeability factor (VPF), platelet-derived endothelial cell growth factor
cell growth factor (PD-ECGF), etc., is also a substance that indirectly acts on vascular endothelial cells.
factor-α (TGF-α), transforming growth factor-β (T
GF-β), angiogenin, tumor necrosis factor-α (TNF-
α) etc. have been found [Folkman, J. & Shing, Y., J.
Biol. Chem., 267: 10931 (1992)].
【0003】これらの中で、VPFに関しては、マウ
ス、ラット、モルモット、ウシおよびヒトの正常または
腫瘍細胞株で分泌されており、また組織別では脳、下垂
体、腎臓、卵巣に存在することが明らかにされている
[(Ferrara,N., et.al. EndocrineReviews 13:18(199
2)]。またヒトVPFは乳癌の血管新生と転移[Weider,
N, et.al. N.Engl.J.Med. 324:1(1991)] や腎細胞癌の
血管新生[医学のあゆみ,168:231(1994)]、あるいは網膜
疾患における血管新生[Adamis,A.P. et.al., Biochem.B
iophys.Res.Comm.,193:631(1993)]に関与していること
が報告されている。ヒトVPF遺伝子についてはそのc
DNAがすでに単離されて塩基配列が決定され、アミノ
酸配列も推定されている。この遺伝子からアミノ酸残基
数の異なる4種類の蛋白(アミノ酸残基数が121個、
165個、189個、206個の4種類)が作られ、そ
れらの中で121個のアミノ酸残基数のもの(VPF12
1)と165個のアミノ酸残基数のもの(VPF165)が成
熟蛋白であると言われている[(Ferrara,N., et.al. End
ocrine Reviews 13:18(1992)]。VPF121はVPF165
のカルボキシル末端の44個のアミノ酸が欠損したもの
であるが、VPF121とVPF165の間に、血管内皮細胞
に対する作用の違いがあるかどうかについては明らかで
ない。このヒトVPF121に対するモノクローナル抗体
はすでに本発明者らにより取得されており、そのモノク
ローナル抗体およびヒトVPF121に対するポリクロー
ナル抗体を用いた酵素免疫測定法によりVPFが測定で
きることを明らかにしている(日本特許:ペプチドおよ
びモノクローナル抗体、出願日平成6年6月10日)。
また、酵素免疫測定法におけるVPFの検出法について
もすでに本発明者らにより確立されており、数pg/mlの
VPFを検出できることを明らかにしている(特願平7
−141271号)。Of these, VPF is secreted in mouse, rat, guinea pig, bovine and human normal or tumor cell lines, and depending on the tissue, it may be present in brain, pituitary gland, kidney and ovary. Has been revealed
[(Ferrara, N., et.al. EndocrineReviews 13:18 (199
2)]. Human VPF is also involved in breast cancer angiogenesis and metastasis [Weider,
N. et.al. N. Engl. J. Med. 324: 1 (1991)] and angiogenesis of renal cell carcinoma [Ayumi, 168: 231 (1994)] or retinal disease [Adamis, AP et.al., Biochem.B
iophys.Res.Comm., 193: 631 (1993)]. C for human VPF gene
DNA has already been isolated, its nucleotide sequence has been determined, and its amino acid sequence has been deduced. 4 kinds of proteins with different number of amino acid residues from this gene (121 amino acid residues,
165, 189, and 206 types) were created, and among them, those with 121 amino acid residues (VPF12
1) and 165 amino acid residues (VPF165) are said to be mature proteins [(Ferrara, N., et.al. End
ocrine Reviews 13:18 (1992)]. VPF121 is VPF165
It has a deletion of the 44 amino acids at the carboxyl terminus, but it is not clear whether VPF121 and VPF165 have different effects on vascular endothelial cells. This monoclonal antibody against human VPF121 has already been obtained by the present inventors, and it has been clarified that VPF can be measured by an enzyme immunoassay using the monoclonal antibody and the polyclonal antibody against human VPF121 (Japanese Patent: Peptide and Monoclonal antibody, filing date June 10, 1994).
In addition, the present inventors have already established a method for detecting VPF in the enzyme immunoassay, and it has been clarified that VPF of several pg / ml can be detected (Japanese Patent Application No. Hei 7).
-141271).
【0004】[0004]
【発明が解決しようとする課題】本発明者らは、以上の
様な知見の基に、腫瘍マーカーとして、特に早期肺癌の
診断のために有用な腫瘍マーカーを見つけるべく鋭意検
討を行ったのである。Based on the above findings, the present inventors have conducted earnest studies to find a tumor marker useful as a tumor marker, particularly for the diagnosis of early lung cancer. .
【0005】[0005]
【課題を解決するための手段】本発明者らは種々検討を
行った結果、上記VPFが腫瘍マーカーとして、特に早
期肺癌の診断のために有用な腫瘍マーカーとして有用な
ものであることを見出し本発明を完成したのである。す
なわち、本発明は、ヒト血清中に存在する血管透過性因
子の存在量に基づくことを特徴とする肺癌細胞の有無判
定方法に関する発明と血管透過性因子の抗体からなるこ
とを特徴とする肺癌診断用検査薬に関する発明からなる
ものである。As a result of various investigations, the present inventors have found that the above VPF is useful as a tumor marker, particularly as a tumor marker useful for diagnosing early lung cancer. The invention was completed. That is, the present invention is an invention relating to a method for determining the presence or absence of lung cancer cells, which is based on the amount of vascular permeability factor present in human serum, and a lung cancer diagnosis characterized by comprising an antibody of vascular permeability factor. The invention relates to an inspection drug for medical use.
【0006】[0006]
【発明の実施の形態】VPFは前記した様にその機能と
ともに公知のものであり、血清中のVPFの存在を確認
する方法としても公知の方法が用いられるが、本発明に
とり好ましい方法は、VPFのポリクローナル抗体また
はモノクローナル抗体を用いる抗原抗体反応、特に標識
免疫測定法、すなわち、赤血球、ラテックス、放射性同
位元素、酵素、発光物質、蛍光物質、金属分子、金属ゲ
ル、バクテリオファージなどを標識として用いる標識免
疫測定法が好ましい。特に、先に本発明者らが特許出願
した化学発光検出系酵素免疫測定法を用いるのが好まし
く、それによれば血清中のVPFを高感度で測定するこ
とが可能になり、肺癌の診断に本発明が特に有用なもの
となる。化学発光検出系酵素免疫測定法は、酵素の基質
として発光基質を用いて発生する光を測定する方法であ
り、VPFに対する抗体を用いるものであり、当該酵素
免疫測定法としては、ヒトVPFに対するモノクローナ
ル抗体やポリクローナル抗体を用いたサンドイッチ法な
どを適用することができる。BEST MODE FOR CARRYING OUT THE INVENTION VPF is known as well as its function as described above, and a known method can be used as a method for confirming the presence of VPF in serum. The preferred method for the present invention is VPF. Antigen-antibody reaction using a polyclonal antibody or a monoclonal antibody, particularly a label immunoassay, that is, a label using erythrocyte, latex, radioisotope, enzyme, luminescent substance, fluorescent substance, metal molecule, metal gel, bacteriophage, etc. as a label Immunoassay methods are preferred. In particular, it is preferable to use the chemiluminescence detection system enzyme immunoassay that the present inventors have previously applied for a patent, which makes it possible to measure VPF in serum with high sensitivity, which is useful for diagnosing lung cancer. The invention becomes particularly useful. The chemiluminescence detection system enzyme immunoassay is a method of measuring light generated by using a luminescent substrate as a substrate of an enzyme, and uses an antibody against VPF, and the enzyme immunoassay is a monoclonal antibody against human VPF. A sandwich method or the like using an antibody or a polyclonal antibody can be applied.
【0007】[0007]
【作用】本発明者らが明らかにしたところによれば、V
PFは、これまで用いられてきた血清中の肺癌マーカー
とは異なり、癌細胞の増殖・進展に必須のものであるた
め、組織型に関わりなくすべて癌細胞において発現が認
められると考えられ、従来のものと異なり、組織型に影
響されることのない早期診断を目的とした血清腫瘍マー
カーとして有用性の高いものであり、さらに、癌細胞の
増殖・進展と密接に関係していることより、治療効果の
判定、経過観察あるいは予後因子としても用いることが
できるという優れた血清腫瘍マーカーとしての作用を示
すものである。According to the clarification by the present inventors, V
Unlike conventional lung cancer markers in serum, PF is essential for the growth and progression of cancer cells, so it is considered that PF is expressed in all cancer cells regardless of tissue type. Unlike that, it is highly useful as a serum tumor marker for the purpose of early diagnosis without being affected by tissue type, and further, because it is closely related to the growth and progression of cancer cells, It exhibits an action as an excellent serum tumor marker that can be used as a therapeutic effect determination, follow-up observation or prognostic factor.
【0008】[0008]
【実施例】以下実施例に基づいて本発明を説明する。 (1)抗VPF ポリクローナル抗体の作製 単離したヒトVPF cDNA をグルタチオン S-トラ
ンスフェラーゼ(GST)との融合蛋白(GST−VPF)
として大腸菌で産生させ、得られた蛋白を抗原として常
法に従ってウサギ抗VPF ポリクローナル抗体を作製
した。抗体価の上昇したウサギの血清を分離し、陰イオ
ン交換カラムクロマトグラフィーによりウサギ抗VPF
ポリクローナル抗体のIgG画分を得た。DESCRIPTION OF THE PREFERRED EMBODIMENTS The present invention will be described below based on embodiments. (1) Preparation of anti-VPF polyclonal antibody Fusion protein (GST-VPF) with isolated human VPF cDNA and glutathione S-transferase (GST)
Was produced in E. coli and the obtained protein was used as an antigen to prepare a rabbit anti-VPF polyclonal antibody according to a conventional method. Rabbit serum with increased antibody titer was isolated and subjected to rabbit anti-VPF by anion exchange column chromatography.
An IgG fraction of the polyclonal antibody was obtained.
【0009】(2)抗VPFポリクローナル抗体の酵素
標識 IgG画分の一部をペプシンで消化してF(ab')2 を調製
後、ヒンジ法によりアルカリフォスファターゼ(ウシ小
腸由来)と結合させ、アルカリフォスファターゼ標識し
たウサギ抗VPFポリクローナル抗体を得た。(2) Enzyme Labeling of Anti-VPF Polyclonal Antibody A part of the IgG fraction was digested with pepsin to prepare F (ab ') 2, which was then bound with alkaline phosphatase (derived from bovine small intestine) by the hinge method to give an alkaline solution. A rabbit anti-VPF polyclonal antibody labeled with phosphatase was obtained.
【0010】(3)肺癌患者血清中VPF濃度の測定 肺癌患者血清中のVPF濃度を以下に示すように、化学
発光検出法を用いた酵素免疫測定法により測定した。抗
VPFポリクローナル抗体(5μg/ml)を 100μl/w
ellずつ96穴プレートにまき4℃で一晩放置した後、
0.1%ウシ血清アルブミン(BSA), PBSで4回洗
浄した。1%BSA、0.1M塩化ナトリウム、0.1%
アジ化ナトリウム、0.2M炭酸ナトリウム緩衝液 pH
9.5でブロッキング(室温で1時間)した後、1%ウシ
血清アルブミン、0.4%ゲラチン、1mM塩化マグネシ
ウム、20mMエチレンジアミン四酢酸ナトリウム、0.
1M塩化ナトリウム、0.1%アジ化ナトリウムを含む
50mMリン酸ナトリウム緩衝液 pH7.0(検体希釈液)
で10倍に希釈した血清(肺癌患者または健常者)あるい
は同検体希釈液に溶解した標準VPFを入れ室温で1時
間放置した。0.05%ツイーン20、0.14M塩化ナ
トリウム、5mM塩化カリウムを含むトリス緩衝液 pH
7.4(TBS−T)で4回洗浄後、アルカリフォスファ
ターゼ標識抗VPFポリクローナル抗体を100μl/w
ellずつ入れ室温で1時間反応させた。TBS−Tで4
回、さらに0.14M塩化ナトリウム、5mM塩化カリウ
ムを含むトリス緩衝液 pH7.4で2回洗浄した後、1m
M塩化マグネシウム、0.02%アジ化ナトリウムを含
む0.1Mジエタノールアミン緩衝液 pH10.0で5倍
に希釈したルミフォス530(和光純薬工業(株)製)を1
00μl/wellずつ入れ、37℃で30分間放置後、発
光強度を測定した。28人の肺癌患者の血清中VPF濃
度の測定結果を、散布図として図1に示した。高値検体
で約300pg/mlであり、平均値は84.7pg/mlであっ
た。一方、健常者290人の血清中VPF濃度を同様に
測定した結果、高値検体で約120pg/ml 程度であり、
平均値は24.9pg/mlであった(図2)。以上のことよ
り、肺癌患者では、健常者に比べて、血清中のVPF濃
度が有意に高いと言える。また、健常者血清中のVPF
濃度の平均値+2倍の標準偏差値をカットオフ値とし
て、肺癌患者での陽性率を計算すると61%であり、血
清診断マーカーとして用いることができるものである。(3) Measurement of VPF concentration in serum of lung cancer patient The VPF concentration in serum of lung cancer patient was measured by enzyme immunoassay using chemiluminescence detection method as shown below. 100 μl / w of anti-VPF polyclonal antibody (5 μg / ml)
Spread each ell on a 96-well plate and leave at 4 ° C overnight,
The plate was washed 4 times with 0.1% bovine serum albumin (BSA), PBS. 1% BSA, 0.1M sodium chloride, 0.1%
Sodium azide, 0.2M sodium carbonate buffer pH
After blocking with 9.5 (1 hour at room temperature), 1% bovine serum albumin, 0.4% gelatin, 1 mM magnesium chloride, 20 mM sodium ethylenediaminetetraacetate, 0.1%.
50mM sodium phosphate buffer containing 1M sodium chloride and 0.1% sodium azide pH 7.0 (specimen diluent)
Serum (lung cancer patient or healthy person) diluted 10-fold with or standard VPF dissolved in the same specimen diluent was added and left at room temperature for 1 hour. Tris buffer pH 0.05% Tween 20, 0.14M sodium chloride, 5 mM potassium chloride
After washing 4 times with 7.4 (TBS-T), 100 μl / w of alkaline phosphatase-labeled anti-VPF polyclonal antibody was used.
Each ell was added and reacted at room temperature for 1 hour. 4 with TBS-T
After washing twice with Tris buffer pH 7.4 containing 0.14M sodium chloride and 5 mM potassium chloride, 1m
Lumiphos 530 (manufactured by Wako Pure Chemical Industries, Ltd.) diluted 5 times with 0.1 M diethanolamine buffer containing 10.0 M magnesium chloride and 0.02% sodium azide was used.
After adding each 00 μl / well and leaving at 37 ° C. for 30 minutes, the emission intensity was measured. The measurement results of the serum VPF concentration of 28 lung cancer patients are shown in FIG. 1 as a scatter diagram. The high value sample was about 300 pg / ml, and the average value was 84.7 pg / ml. On the other hand, as a result of measuring the VPF concentration in serum of 290 healthy subjects in the same manner, it was about 120 pg / ml in the high value sample,
The average value was 24.9 pg / ml (Fig. 2). From the above, it can be said that lung cancer patients have significantly higher VPF concentration in serum than healthy subjects. In addition, VPF in serum of healthy subjects
The positive rate in lung cancer patients was calculated to be 61% using the cutoff value as the average value of the concentration plus twice the standard deviation value, which can be used as a serum diagnostic marker.
【0011】[0011]
【発明の効果】本発明者らが見出した血清中の肺癌マー
カーとして優れるVPFは、これを測定することによ
り、特に化学発光検出系酵素免疫測定法を用いて高感度
で測定することにより、肺癌の早期診断、さらには治療
効果の判定、経過観察に非常に有用に用いられるもので
ある。INDUSTRIAL APPLICABILITY The VPF, which was found by the present inventors and is excellent as a lung cancer marker in serum, can be determined by measuring it, particularly by using a chemiluminescence-detecting enzyme immunoassay with high sensitivity. It is very useful for the early diagnosis of, the determination of the therapeutic effect, and the follow-up observation.
【図1】化学発光検出系を用いた酵素免疫測定法によ
り、肺癌患者血清検体28例の血清中VPF量の測定結
果の散布図である。FIG. 1 is a scatter diagram of the measurement results of the amount of VPF in serum of 28 serum samples of lung cancer patients by an enzyme immunoassay using a chemiluminescence detection system.
【図2】化学発光検出系を用いた酵素免疫測定法によ
り、健常者血清検体290例の血清中VPF量の測定結
果の散布図である。FIG. 2 is a scatter diagram of the measurement results of the amount of VPF in serum of 290 healthy human serum samples by an enzyme immunoassay using a chemiluminescence detection system.
Claims (2)
在量に基づくことを特徴とする肺癌細胞の有無判定方
法。1. A method for determining the presence or absence of lung cancer cells, which is based on the amount of vascular permeability factor present in human serum.
とする肺癌診断用検査薬。2. A diagnostic agent for diagnosing lung cancer, which comprises an antibody of a vascular permeability factor.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP20665995A JPH0933531A (en) | 1995-07-20 | 1995-07-20 | Method for deciding presence of lung cancer cell and examination medicine for diagnosing lung cancer |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP20665995A JPH0933531A (en) | 1995-07-20 | 1995-07-20 | Method for deciding presence of lung cancer cell and examination medicine for diagnosing lung cancer |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| JPH0933531A true JPH0933531A (en) | 1997-02-07 |
Family
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Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| JP20665995A Pending JPH0933531A (en) | 1995-07-20 | 1995-07-20 | Method for deciding presence of lung cancer cell and examination medicine for diagnosing lung cancer |
Country Status (1)
| Country | Link |
|---|---|
| JP (1) | JPH0933531A (en) |
Cited By (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN102937649A (en) * | 2012-10-18 | 2013-02-20 | 上海交通大学 | Miniaturized magnetic fluxgate biosensor for serum tumor marker detection |
-
1995
- 1995-07-20 JP JP20665995A patent/JPH0933531A/en active Pending
Cited By (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN102937649A (en) * | 2012-10-18 | 2013-02-20 | 上海交通大学 | Miniaturized magnetic fluxgate biosensor for serum tumor marker detection |
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