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생물학적 설명

특이성	GNA13 Antibody [P10C14]는 총 GNA13 단백질의 내인성 수준을 인식합니다.
배경	GNA13(구아닌 뉴클레오타이드 결합 단백질 서브유닛 알파-13)은 GNA13 유전자에 의해 암호화되는 필수 단백질이며, 이형삼량체 G 단백질 계열에 속합니다. 이는 성장, 분화 및 운동성을 포함한 다양한 세포 기능에 필수적인 G 단백질 결합 수용체(GPCR)로부터 신호를 전달하는 데 중요한 역할을 합니다. GNA13은 GTP에 결합했을 때 주로 활성화되며, 이는 ARHGEF1과 같은 하류 이펙터와 상호작용하여 Rho GTPase를 활성화하여 액틴 세포골격을 조절합니다. 이 단백질은 림프계 및 혈관계를 포함한 다양한 조직에서 발현되며, 혈관신생, 여성 생식능력 및 뼈 항상성을 포함한 여러 생리적 과정에 관여합니다. GNA13 유전자의 돌연변이는 미만성 거대 B세포 림프종(DLBCL), 특히 배중심 B세포 유사 아형과 관련이 있습니다. 이러한 돌연변이는 세포 생존 및 증식을 향상시키는 기능 상실 효과를 초래하며, 이는 GNA13의 종양 억제자 역할을 시사합니다.

특이성

GNA13 Antibody [P10C14]는 총 GNA13 단백질의 내인성 수준을 인식합니다.

배경

GNA13(구아닌 뉴클레오타이드 결합 단백질 서브유닛 알파-13)은 GNA13 유전자에 의해 암호화되는 필수 단백질이며, 이형삼량체 G 단백질 계열에 속합니다. 이는 성장, 분화 및 운동성을 포함한 다양한 세포 기능에 필수적인 G 단백질 결합 수용체(GPCR)로부터 신호를 전달하는 데 중요한 역할을 합니다. GNA13은 GTP에 결합했을 때 주로 활성화되며, 이는 ARHGEF1과 같은 하류 이펙터와 상호작용하여 Rho GTPase를 활성화하여 액틴 세포골격을 조절합니다. 이 단백질은 림프계 및 혈관계를 포함한 다양한 조직에서 발현되며, 혈관신생, 여성 생식능력 및 뼈 항상성을 포함한 여러 생리적 과정에 관여합니다. GNA13 유전자의 돌연변이는 미만성 거대 B세포 림프종(DLBCL), 특히 배중심 B세포 유사 아형과 관련이 있습니다. 이러한 돌연변이는 세포 생존 및 증식을 향상시키는 기능 상실 효과를 초래하며, 이는 GNA13의 종양 억제자 역할을 시사합니다.

사용 정보

응용

WB, IHC

희석

WB	IHC
1:1000-1:10000	1:1000

반응성

Human, Mouse, Rat

출처

Rabbit Monoclonal Antibody

MW

44 Kda

보관 완충액

PBS, pH 7.2+50% Glycerol+0.05% BSA+0.01% NaN₃

보관
(수령일로부터)

-20°C (avoid freeze-thaw cycles), 2 years

실험 방법
WB	Experimental Protocol: Sample preparation 1. Tissue: Lyse the tissue sample by adding an appropriate volume of ice-cold RIPA/NP-40 Lysis Buffer (containing Protease Inhibitor Cocktail)，and homogenize the tissue at a low temperature or lyse it by sonication on ice, then incubate on ice for 30 minutes. 2. Adherent cell: Aspirate the culture medium and transfer the cells into an EP tube. Wash the cells with ice-cold PBS twice. Add an appropriate volume of RIPA/NP-40 Lysis Buffer (containing Protease Inhibitor Cocktail), sonicate to lyse the cells, and incubate on ice for 30 minutes. 3. Suspension cell: Transfer the culture medium to a pre-cooled centrifuge tube. Centrifuge and aspirate the supernatant. Wash the cells with ice-cold PBS twice.Add an appropriate volume of RIPA/NP-40 Lysis Buffer (containing Protease Inhibitor Cocktail), sonicate to lyse the cells, and incubate on ice for 30 minutes. 4. Place the lysate into a pre-cooled microcentrifuge tube. Centrifuge at 4°C for 15 min. Collect the supernatant; 5. Remove a small volume of lysate to determine the protein concentration; 6. Combine the lysate with protein loading buffer. Boil 20 µL sample under 95-100°C for 5 min. Centrifuge for 5 min after cool down on ice. Electrophoretic separation 1. According to the concentration of extracted protein, load appropriate amount of protein sample and marker onto SDS-PAGE gels for electrophoresis. Recommended separating gel (lower gel) concentration: 10%. Reference Table for Selecting SDS-PAGE Separation Gel Concentrations 2. Power up 80V for 30 minutes. Then the power supply is adjusted (110 V~150 V), the Marker is observed, and the electrophoresis can be stopped when the indicator band of the predyed protein Marker where the protein is located is properly separated. (Note that the current should not be too large when electrophoresis, too large current (more than 150 mA) will cause the temperature to rise, affecting the result of running glue. If high currents cannot be avoided, an ice bath can be used to cool the bath.) Transfer membrane 1. Take out the converter, soak the clip and consumables in the pre-cooled converter; 2. Activate PVDF membrane with methanol for 1 min and rinse with transfer buffer; 3. Install it in the order of "black edge of clip - sponge - filter paper - filter paper - glue -PVDF membrane - filter paper - filter paper - sponge - white edge of clip"; 4. The protein was electrotransferred to PVDF membrane. ( 0.45 µm PVDF membrane is recommended ) Reference Table for Selecting PVDF Membrane Pore Size Specifications Recommended conditions for wet transfer: 200 mA, 120 min. ( Note that the transfer conditions can be adjusted according to the protein size. For high-molecular-weight proteins, a higher current and longer transfer time are recommended. However, ensure that the transfer tank remains at a low temperature to prevent gel melting.) Block 1. After electrotransfer, wash the film with TBST at room temperature for 5 minutes; 2. Incubate the film in the blocking solution for 1 hour at room temperature; 3. Wash the film with TBST for 3 times, 5 minutes each time. Antibody incubation 1. Use 5% skim milk powder to prepare the primary antibody working liquid (recommended dilution ratio for primary antibody 1:1000), gently shake and incubate with the film at 4°C overnight; 2. Wash the film with TBST 3 times, 5 minutes each time; 3. Add the secondary antibody to the blocking solution and incubate with the film gently at room temperature for 1 hour; 4. After incubation, wash the film with TBST 3 times for 5 minutes each time. Antibody staining 1140. Add the prepared ECL luminescent substrate (or select other color developing substrate according to the second antibody) and mix evenly; 2. Incubate with the film for 1 minute, remove excess substrate (keep the film moist), wrap with plastic film, and expose in the imaging system.
IHC	Experimental Protocol： Deparaffinization/Rehydration 1. Deparaffinize/hydrate sections: 2. Incubate sections in three washes of xylene for 5 min each. 3. Incubate sections in two washes of 100% ethanol for 10 min each. 4. Incubate sections in two washes of 95% ethanol for 10 min each. 5. Wash sections two times in dH2O for 5 min each. 6.Antigen retrieval: For Citrate: Heat slides in a microwave submersed in 1X citrate unmasking solution until boiling is initiated; continue with 10 min at a sub-boiling temperature (95°-98°C). Cool slides on bench top for 30 min. Staining 1. Wash sections in dH2O three times for 5 min each. 2. Incubate sections in 3% hydrogen peroxide for 10 min. 3. Wash sections in dH2O two times for 5 min each. 4. Wash sections in wash buffer for 5 min. 5. Block each section with 100–400 µl of blocking solution for 1 hr at room temperature. 6. Remove blocking solution and add 100–400 µl primary antibody diluent in to each section. Incubate overnight at 4°C. 7. Remove antibody solution and wash sections with wash buffer three times for 5 min each. 8. Cover section with 1–3 drops HRPas needed. Incubate in a humidified chamber for 30 min at room temperature. 9. Wash sections three times with wash buffer for 5 min each. 10. Add DAB Chromogen Concentrate to DAB Diluent and mix well before use. 11. Apply 100–400 µl DAB to each section and monitor closely. 1–10 min generally provides an acceptable staining intensity. 12. Immerse slides in dH2O. 13. If desired, counterstain sections with hematoxylin. 14. Wash sections in dH2O two times for 5 min each. 15. Dehydrate sections: Incubate sections in 95% ethanol two times for 10 sec each; Repeat in 100% ethanol, incubating sections two times for 10 sec each; Repeat in xylene, incubating sections two times for 10 sec each. 16. Mount sections with coverslips and mounting medium.

참조

https://pubmed.ncbi.nlm.nih.gov/33423045/

적용 데이터

WB

Selleck 검증

Lane 1 : HepG2
Lane 2 : 293T
Lane 3 : HepG2
Lane 4 : Mouse brain
Lane 5 : Rat brain