SKU: 13233177021

Rat ACTH ELISA Kit

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Description

Rat ACTH ELISA KitProduct Specification protein ACTH Usage Sample collection preparation and preservation 1. Serum: Whole blood sample placed at room temperature 2 Hour or 4C After overnight 1000g Centrifugation 20 Minutes, take the supernatant to detect. The blood collection tubes shall be disposable non pyrogenic, non endotoxin tubes. deposit 20C Or 80C Storage, avoid repeated freezing and thawing. 2. Plasma: the sample after collection 30 Within minutes 2 8C 1000g

Product Specification

protein ACTH
Usage

Sample collection preparation and preservation


1. Serum: Whole blood sample placed at room temperature 2 Hour or 4°C After overnight 1000×g Centrifugation 20 Minutes, take the supernatant to detect. The blood collection tubes shall be disposable non-pyrogenic, non-endotoxin tubes. deposit -20°C Or -80°C Storage, avoid repeated freezing and thawing.


2. Plasma: the sample after collection 30 Within minutes 2-8°C 、 1000×g Centrifugation 15 Minutes, take the supernatant to detect. Anticoagulants recommended EDTA-Na2 , avoid using hemolytic, hyperlipidemic samples. deposit -20°C Or -80°C Storage, avoid repeated freezing and thawing.


3. Tissue homogenate: Take an appropriate amount of tissue block and add it to the pre-cooled PBS ( 0.01M , pH7.0-7.2 ) to remove blood (lysed red blood cells in the homogenate will affect the measurement result), cut the tissue into pieces after weighing, and then mix it with the corresponding volume of PBS (generally according to 1:9 The mass-to-volume ratio, the specific volume can be appropriately adjusted according to the needs of the experiment, and recorded. It is recommended to PBS Adding a protease inhibitor) into a glass homogenizer and fully grinding on ice; In order to further lyse tissue cells, the homogenate can be subjected to ultrasonic disruption or repeated freeze-thaw treatment (pay attention to ice bath cooling during ultrasonic disruption, and the repeated freeze-thaw method can be repeated 2 Times). Finally, the prepared homogenate is mixed in 5000×g Centrifugation 5-10 Minutes, take the supernatant to detect. (Tissue homogenates require simultaneous detection of protein concentrations to obtain a more accurate test substance concentration per milligram of protein.)


4. Cell culture supernatant: Take the cell supernatant from 1000×g Centrifugation 20 Minutes, impurities and cell debris were removed. Take the supernatant to detect and place it in -20°C Or -80°C Store, but repeated freezing and thawing should be avoided.


5. Urine: Please collect the first urine in the morning (mid-section urine), or 24 Hourly urine, 2000×g Centrifugation 15 The supernatant was collected after minutes and the sample was saved At -20°C And repeated freezing and thawing should be avoided.


6. Saliva: A sample is collected with a saliva sample collection tube, and then 2-8°C, 1000×g Centrifugation 15 Minutes, take the supernatant to detect, or sub-package -20°C Save. Avoid repeated freezing and thawing.


7. Other biological samples: Please 1000×g Centrifugation 20 Minutes, take the supernatant to detect.

Notes


1. The sample should be clear and transparent, and the suspended solids should be removed by centrifugation. Hemolysis of the sample will affect the results, so hemolyzed samples should not be used.


2. After sample collection, if 1 Testing within weeks can be stored at 4°C , if it cannot be detected in time, please pack it according to the one-time usage amount and freeze it in -20°C ( 1 Within months), or -80°C ( 3-6 Test within a month) to avoid repeated freezing and thawing. Keep the sample at room temperature prior to the experiment.

Principles of sample dilution


If your test sample needs to be diluted, refer to the general dilution principles below:


1. Dilution 50 Times: One-step dilution. Take 5 μL Sample to 245 μL Standard & In the sample dilution, is 50 Double dilution;


2. Dilution 100 Times: One-step dilution. Take 5 μL Sample to 495 μL Standard & In the sample dilution, is 100 Double dilution;


3. Dilution 1000 Times: Two-step dilution. Take 5 μL Sample to 95 μL Standard & In the sample dilution, is 20 Dilute, and then take 5 μL 20 Double dilute sample to 245 μL Standard & In the sample dilution, is 50 Double dilution, co-dilution 1000 Times;


4. Dilution 100000 Times: Three-step dilution. Take 5 μL Sample to 195 μL Standard & In the sample dilution, is 40 Dilute, and then take 5 μL 40 Double dilute sample to 245 μL Standard & In the sample diluent, do 50 Time dilution, and finally take 5 μL 2000 Double dilute sample to 245 μL Standard & In the sample diluent, do 50 Double dilution, total dilution 100000 Times;


5. The amount of liquid taken during each dilution step is not less than 3 μL , the dilution factor is not more than 100 Times. Too small sampling volume can easily cause greater errors in the mixing process, and each step of dilution needs to be mixed evenly to avoid foaming.


6. When the dilution factor is very high, you can use it first PBS Dilution, last step using standard in kit & Sample dilution.


Sample dilution recommendations


1. Normal fresh serum / Plasma Sample Recommendation (Original solution-1:5) Testing.


2. Due to individual variations, the recommended dilution factor is for informational purposes only. For actual testing, please estimate the concentration range of the sample in advance, and determine the dilution factor of the sample to be tested through pre-experiments.

Preparation for testing


1. Please advance 30 Minutes remove the kit from the refrigerator and equilibrate to room temperature.


2. Use double distilled water 25× The concentrated wash liquid is diluted to 1× Working fluid, put back unused 4°C 。


3. Standard: Add standard & Sample Universal Diluent 1.0 mL Into the lyophilized standard, screw the tube cap tightly and let stand 10 Minutes, and after it is fully dissolved, gently mix (concentration of 2000 pg/mL )。 Thereafter, double dilution is carried out to 2000 pg/mL , 1000 pg/mL , 500 pg/mL , 250 pg/mL , 125 pg/mL , 62.5 pg/mL , 31.25 pg/mL Standard dilution ( 0 pg/mL ) is a blank hole. Configure the standard according to the amount you need for later use. The configured standards are recommended in 15 Add the sample within minutes, and it is not recommended to leave it for too long.


4. Biotinylated antibody working solution: calculate the dosage required for the current experiment before the experiment (according to 100 μL/ Hole meter, should be configured more in actual configuration 100-200 μL ), before use 15 Min, concentrated biotinylated antibody was diluted with biotinylated antibody diluent ( 1:100 ) into working concentration, use on the same day. Dilution principle 1 μL Concentrated biotinylated antibody is added to 99 μL In the biotinylated antibody dilution, mix well with a pipette.


5. Enzyme conjugate working solution: calculate the dosage required for the current experiment before the experiment (according to 100 μL/ Hole meter, should be configured more in actual configuration 100-200 μL )。 Before use 15 Minutes, dilute and concentrate with enzyme conjugate diluent HRP Enzyme conjugate ( 1:100 ) into working concentration, use on the same day. Dilution principle 1 μL The concentrated enzyme conjugate is added to 99 μL The enzyme conjugate dilution was mixed with a pipette.


6.TMB Substrate —— Pipette the desired dose of solution and do not pour the residual solution back into the reagent vial again.


Preparation before the experiment


1. All materials and prepared reagents were equilibrated to room temperature prior to use. Before use, mix all reagents thoroughly, taking care not to create any foam.


2. The user should calculate the number of samples that may be used throughout the trial. Please reserve enough samples in advance.


3. Please estimate the concentration before measurement. If these values are not within the standard curve range, the user must determine the optimal sample dilution for their particular experiment.

Operation steps


1. Before the start of the experiment, each reagent should be balanced to room temperature, and all reagents should be configured in advance. When reagents or samples are diluted, they should be mixed evenly, and foaming should be avoided as much as possible when mixing evenly. If the sample concentration is too high, dilute with a sample diluent to bring the sample within the range of the kit.


2. Add standard or sample to be tested 100 μL (If the sample needs to be diluted, please refer to the sample dilution principle for the dilution method). Be careful not to have bubbles. When adding the sample, add the sample to the bottom of the well of the enzyme label plate, try not to touch the well wall, gently shake and mix well, and add the enzyme label plate. Cover or coating, 37°C incubation 80 Minutes. To ensure the validity of the experimental results, please use a new standard solution for each experiment.


3. Discard the liquid in the hole, spin dry, wash the plate 3 Times. For each well 200 μL Washing with washing solution, soaking 1-2 Minutes, shake off the liquid in the labeled plate (or wash the plate with a plate washer). After the last wash was complete, the plate was pat dry on absorbent paper.


4. Add biotin antibody working solution per well 100μL (can be advanced 15 Preparation in minutes), the enzyme labeled plate is coated, 37°C incubation 50 Minutes.


5. Discard the liquid in the well and wash the plate 3 Times. For each well 200μL Washing with washing solution, soaking 1-2 Minutes, shake off the liquid in the labeled plate (or wash the plate with a plate washer). After the last wash was complete, the plate was pat dry on absorbent paper.


6. Add enzyme conjugate working solution per well 100 μL (can be advanced 15 Minute preparation), 37°C incubation 50 Minutes.    


7. Discard the liquid in the well and wash the plate 5 Times. For each well 200 μL Washing with washing solution, soaking 1-2 Minutes, shake off the liquid in the labeled plate (or wash the plate with a plate washer). After the last wash was complete, the plate was pat dry on absorbent paper.


8. Add per well TMB Chromogenic substrate solution 90 μL , 37°C Incubate in the dark 20 Minutes (shortened or extended as appropriate according to the actual color development, but not exceeding 30 Minutes).


9. Add stop solution to each well 50 μL , terminate the reaction (blue immediately turns yellow at this time). The sequence of addition of the terminating solution should be the same as that of the developer as possible. In order to ensure the accuracy of the experimental results, the termination solution should be added as soon as possible after the substrate reaction time expires.


10. Immediately use a microplate reader in 450 nm The optical density values of each well were measured at the wavelength ( OD Value). The instrument should be preheated before use, and the testing program should be set up.

Results Calculation


1. Of each standard and sample OD Value should be subtracted from the blank hole OD Value. If a double hole is set, the average value should be taken for calculation.


2. For ease of calculation, although the concentration is an independent variable and OD The value is the dependent variable, and we still use the standard when drawing OD Values as abscissa ( X Axis), the concentration of the standard is the ordinate ( Y Axis). At the same time, for the intuition of the test results, the figure provides raw data instead of logarithmic values. Due to the different experimental operating conditions ( such as operator, pipetting technology, plate washing technology and temperature conditions, etc.), the standard curve OD Values will vary. The standard curve provided is for reference only, and the experimenter needs to establish the standard curve according to his own experiment. Spent sample OD The value can be calculated on the standard curve to calculate the sample concentration and multiply it by the dilution factor, which is the actual concentration of the sample. It is recommended to use professional curve drawing software such as curve expert 。

 

Concentration (pg/mL)

OD

Corrected OD

2000

2.058

1.955

1000

1.585

1.482

500

1.111

1.008

250

0.813

0.71

125

0.591

0.488

62.5

0.364

0.261

31.25

0.261

0.158

0

0.103

0.000


Note : This picture is for reference only

 

Precision


Intraplate precision ( Precision within the assay ):CV%<8%


Three samples with known concentrations were respectively in 1 Test on enzyme label plates 20 Times to evaluate the precision in the assay plate.


Inter-plate precision ( Measure inter-plate precision ):CV%<10%


Three samples with known concentrations were respectively in 3 Tested on different enzyme plates 40 Times to evaluate the precision of the analytical plate.

 

Recovery


Add known concentrations of rats to different samples ACTH , do the recovery experiment, get the recovery range and average recovery rate

Sample Type

Recovery Range

Average recovery

Serum (n=5)

86-99%

92%

EDTA  Plasma (n=5)

89-103%

96%

heparin Plasma (n=5)

83-97%

90%

 

linear


Rats will be added ACTH The samples were diluted separately 2 Times, 4 Times, 8 Times, 16 Double the recovery experiment to obtain the recovery rate range

Sample Type

1:2

1:4

1:8

1:16

Serum (n=5)

92-104%

87-96%

87-99%

96-107%

EDTA  Plasma (n=5)

93-105%

79-86%

87-103%

85-97%

heparin Plasma (n=5)

86-105%

98-107%

90-99%

88-97%

Sensitivity 7.3 pg/mL
Species Reactivity Rat
Theory This kit adopts the principle of sandwich method. The specific anti-rat ACTH antibody was coated in a 96-well microplate, and the rat ACTH standard or sample was added to the microwells respectively, and the rat ACTH protein in the standard or the rat ACTH protein in the sample was bound to the anti-rat ACTH antibody solid on the microplate, then the biotinylated anti-rat ACTH antibody was added, the unbound biotinylated antibody was washed, HRP-labeled streptavidin was added, and the TMB substrate was added to develop color. TMB is converted to blue under peroxidase catalysis and to final yellow under the action of acid. There is a positive correlation between the depth of color and rat ACTH protein in the sample. The absorbance (OD value) was measured with a microplate reader at a wavelength of 450 nm, and the sample concentration was calculated by drawing a standard curve.
Source Rat
Synonym Corticotropin; Adrenocorticotropin;Rat ACTH(Adrenocorticotropic Hormone) ELISA Kit
Detection Type Rat ACTH can be detected in samples and does not cross-react with other related proteins
Composition

Chinese Name

96T

Preservation conditions

Enzyme labeled plate (detachable)

12 Strip x 8 Hole

4°C/-20°C

Lyophilized Standard

2

4°C/-20°C

Standard & Sample dilution

20 mL

4°C/-20°C

Concentrated biotinylated antibodies ( 100× )

120 μL

4°C/-20°C

Biotinylated antibody dilution

12 mL

4°C/-20°C

concentrate HRP Enzyme conjugate ( 100× )

120 μL

4°C/-20°C

Enzyme conjugate dilution

12 mL

4°C/-20°C

Concentrated wash ( 25× )

20 mL

4°C/-20°C

Chromogenic substrate solution ( TMB )

10 mL

4°C/-20°C( Protected from light)

Reaction stop solution

6 mL

4°C/-20°C

Sealing film

2

normal temperature

General Notes

1. Please make sure that all components are dissolved and mixed before using the kit. If the reconstituted standard is not used, please discard it.

2. Concentrate the biotinylated antibody. The volume of the concentrated enzyme conjugate is small and may be dispersed in various parts of the tube during transportation. Please centrifuge at 1000 × g for 1 minute before use, so that the liquid on the tube wall or bottle cap can be deposited to the bottom of the tube. Mix the solution by carefully pipetting 4-5 times with a pipette before taking. Standard, biotinylated antibody working solution and enzyme conjugate working solution should be prepared according to the required dosage, and the corresponding diluent should be used to prepare without confusion.

3. The concentrated washing liquid taken out of the refrigerator may have crystals, which is a normal phenomenon. The crystals can be completely dissolved in a water bath or incubator before preparing the washing liquid (the heating temperature should not exceed 40 °C). The wash liquid should be at room temperature when used.

4. Sample addition needs to be quick, and it is best to control each sample addition within 10 minutes. In order to ensure the accuracy of the experiment, it is recommended to use double holes. Maintaining a consistent sequence of addition from well to well when pipetting reagents will ensure the same incubation time for all wells.

5. During the washing process, the washing liquid remaining in the reaction hole should be patted dry on absorbent paper. Do not put the filter paper directly into the reaction hole to absorb water. Before reading, pay attention to removing the residual liquid and fingerprints at the bottom, so as not to affect the reading of the microplate reader.

6. The developer TMB should avoid direct exposure to strong light during storage and use. After adding the substrate, pay attention to the color change in the reaction well. If the gradient is obvious, please terminate the reaction in advance to avoid too dark color affecting the reading of the microplate reader.

7. The test tubes and reagents used during the experiment are disposable, and it is strictly forbidden to reuse them, otherwise the experimental results will be affected.

8. Please wear a laboratory coat and latex gloves for protection during the experiment, especially when testing blood or other body fluid samples, please follow the national biological laboratory safety protection regulations.

9. Kit components of different batch numbers cannot be mixed (except washing solution and reaction stop solution).

10. The enzyme labeling strip in the kit is a detachable plate, please use it in batches according to the experimental requirements.

Storage Temp. Unopened kit, stored at 2-8 °C, shelf life 6 months.
Test Range 31.25-2000 pg/mL
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this book set my soul ablaze! <3
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"i had never really cared about the weather before, but now, clear skies meant everything to me, and i was grateful to see another calm morning." this book. this book! i loved the last storm so much. the writing style. the descriptions. the world-building. the characters. the plot twists. the tropes. the sexual tension. the—everything. everything was magic. the last storm follows our two main characters, ara and rogue, giving us dual POV from both characters (which i loved, btw). ara, a human girl who has been locked away in her father’s estate most of her life, just wants to see the world. all she dreams of is seeing what else is out there. but when her father announces her engagement, she knows that dream will become nothing more than just that—a dream. rogue, the fae king, is tired of the attacks being rained down on his people. in hopes of finding out the human king adon’s secrets, rogue infiltrates auryna’s borders. in his last resort to gain information, he visits the local pub. to his surprise, the general’s precious only child is sitting at the bar, drink round after round of mead. now he just needs to figure out how to take her without anyone noticing. first and foremost, let’s talk about the endless list of my favorite tropes and aspects that this book had. ›› enemies to lovers ›› fated mates ›› one bed ›› the chosen one ›› elemental magic ›› actually good and shocking plot twists!!! ›› badass female lead ›› morally-grey love interest ›› fae/human war ›› force proximity ›› touch her and die ›› who did this to you? ›› captor/captive ›› praise k!nk (panting profusely) “you are entirely the opposite of everything that i am, and i would gladly wear your shackles if it meant i could have you.” it’s been a long while since i read a book i liked this much. but i just loved this book. it set my soul ablaze. thank you to the author for writing this beautiful story and for blessing me with an eARC! i loved it so much that i immediately bought the paperback upon release! every aspect of this book was just beautiful. i was blown away by the way the world was described, the way feelings were portrayed, the way the elements were used in the fae’s magic. it just—AHHH! i just absolutely adored it all. i cannot wait for the second book to release next year! also the way he calls her “little storm” sets my heart on fire. this was a fast-paced read and if you are a lover of acotar, fbaa, deal with the elf king, or any other similar books, then please stop everything you’re doing and read this book right now. you won’t regret it. thank you again, jd linton, for giving me the privilege of reading your arc and for blessing this world with the world you created. <3 "something about him pulled me in, like a moth to a flame, and it felt as if i was just waiting for the inevitable burn that came with flying too close to the fire."
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Only my second first person written selection, I am still getting used to that aspect, but unlike my first, I enjoyed that the story was told through both MCs. A great enemies to lovers, forced proximity, fated love etc, that resonated to me. There were some small twists that I could see coming, but also a few that I didn’t quite see until the characters were also seeing. Personally, I am more interested in the story than the spice, but with that said, it was well seasoned! I am kind of new to the spice world so I can’t say for sure how this would rate, but it definitely had some heat. I am very glad I happened across this author, and I do plan on also reading the next book….if nothing else, just to see for myself the “transformation” of the characters I’ve grown to love!
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I’m having trouble finding accurate words to describe the way this book made me feel, but I am going to do my best. To start off with basic elements, the character and world building are phenomenal. I feel a strong bond to not only the two main characters, Ara and Rogue, but to each and every character introduced throughout the book. The author did a stellar job of giving each of them unique personhood. All of the scenes are beautifully described. So much so that throughout the entirety of the book, I could see every scene: the towns, the castles, the meadows, the landscape. I have had difficulty with this and with distinguishing between outlying characters while reading in the past, but I did not have to think to remember details of world or character building because they flowed naturally within the story and were described well. I have read book series before that made me want to be a part of that world, but I actually felt like I got to step into Auryna and Ravaryn! The plot twists!! Although this is not a suspense novel, it still had me on a rollercoaster of emotions and on the edge of my seat from beginning to end. I haven’t cried actual tears over a book since I was in high school (and I’ve read a LOT). This book finally broke the floodgates in the final few chapters. Multiple times. And we love a good cliffhanger. It truly made me FEEL. THE SPICE is a solid 3.5/5. Some of the scenes had me flushed, some had me taking notes, some just had my jaw slack and my mouth hanging open. Bravo, JD Linton, bravo. The relationships: friendships, family, romantic, ALL of the relationships in this book have so much meaning. The author does a great job at making you feel the love, the anger, the peace, the frustrations, the safety, the familiarity, etc. between the characters. Ara and Rogue. I can not say enough and I also do not want to say too much. Just know that I feel like I know them both, to their core. I know what their childhood looks likes, their darkest moments, their biggest fears, their dreams and passions, what they want in life… The POV switches were seamless. I am so happy this author decided to let us see from both sets of eyes. I can not wait for book two after that cliffhanger. And there is SO much potential for at least one prequel, I can’t wait to see where this author goes! I hope this series continues and flourishes. Fingers crossed!
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Tracy and Christina
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Amazing!
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This book was phenomenal, I devoured it within a few days! For this being a debut novel, it is fantastic and I would’ve thought the author was a seasoned author. I have zero complaints about this book. Let me start by saying that the world building was phenomenal. I could picture everything in my head because of how detailed it was — that’s how good it was written. And I absolutely love the “captive/captor” trope so much, it’s become one of my favorite tropes, so I was pleasantly surprised to see that this book had that. I loved the banter between Rogue and Ara — they’re both snarky and witty, plus with the romantic tension, it made the dialogue that much better. Speaking of romantic tension, yes there is spice but not so much of it that it overrides the plot, which I loved. For me, this would probably be on the 3/5 level of spice. This book had a ton of plot twists and I thoroughly enjoyed it.
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This is a great Romantasy book full of action, adventure, and everything you look for in this genre. I won’t lie: it does kinda feel like the author found every common trope from every successful book of this kind and threw them all into this novel. But if it ain’t broke, don’t fix it. Especially in romance, there’s a large audience who has specific expectations, and they want them every time. Nothing wrong with that and many times I’m one of them. I have no idea what defines a spoiler honestly, so spoiler alert!!!!!!! Tropes include: Only one bed at the inn/bar Dissatisfaction with life before hunk appears Lost royalty The chosen one Montage of dress up time followed by shocked hunk Forbidden romance between two from rival peoples Power that cannot be controlled, simply guided/asked Gathering intel at the inn/bar FMC who knows how to fight/use weapons well There’s probably more but no need to list them all. Good story and I would recommend!
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Reviewed in the United States on June 14, 2024

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