Jess

Your Complete Protein Analysis Solution

Jess automates the protein separation and immunodetection of traditional Western blotting, eliminating many of the tedious, error-prone steps. Just load your samples and reagents into the microplate and Jess separates your proteins by size, and precisely manages antibody additions, incubations, washes and even the detection steps. Come back to fully analyzed results in 3 hours. Go further with multiplexing—her fluorescent detection gets all the information you need in one shot. Jess, she's like Western blot meets ELISA in one.

Jess

How Can Jess Help You?

I need fast results

With Jess, it's pipette, run & done! Simply load your sample, antibodies and reagents into the plate, insert your plate and cartridge into Jess and press start. All assay steps from protein separation, immunoprobing, detection and analysis of data are fully automated. With just 30 minutes of experimental setup and 3 hours of hands-free run time, you can be analyzing data for your next publication or grant.

Get fast results with Jess

I want to boost my throughput

Got a lot of samples? Jess can dramatically increase your throughput. She automates the protein separation and immunodetection of traditional Western blotting, giving you fully analyzed results in just 3 hours. Everything happens inside a capillary, and Jess precisely controls the protein separation and reagent additions and incubations, even the detection. Use Jess's fluorescent capabilities and multiplex your proteins for even higher throughput. With her 13 and 25 sample capillary cartridges you'll get the throughput you need, with minimum hands-on time.

Boost your throughput with Jess

I want immunoassay-like quantitation from my Westerns

Stop, analyze and wow! With Jess, protein quantitation is a breeze. At the conclusion of your run, use the lane view option to compare band intensity or dive deep for fully quantitative analysis of protein size and concentration. With a few clicks you'll be analyzing immunoassay-like standard curves and precisely quantifying your protein. Multiplexing takes your options to the max, helping you identify and differentiate relative protein expression between samples in one shot. And with in-built protein normalization, you'll have the confidence you need in your results, experiment after experiment.

Quantitate your Westerns with Jess

I want more data per sample

Do traditional assays use too much of your precious samples or require you to pool your samples? Jess gets you down to picogram-level sensitivity with just 3 µL of starting material. Tired of stripping and reprobing? Jess's fluorescent detection lets you maximize the data you get in one shot. Let your sample go further with Jess.

Get more data per sample with Jess

I need to run traditional Westerns, sometimes

Still doing traditional Westerns? Snap! Get the picture with her chemiluminescent blot imaging system.

Chemiluminescent blot imaging with Jess

How Does Jess Work?

Simple Western assays are automated, capillary-based immunoassays that solve many of the challenges that come with traditional Westerns. All assay steps from protein separation, immunoprobing, detection and analysis of data are fully automated. Variability in the manual processes that used to impact reproducibility, quantitation, time to result and overall data reliability is eliminated. Best of all, the transition is simple—the same antibodies you use for Western blotting protocols can be used with Simple Western assays.

Jess gives you four different ways to analyze proteins.

  1. Fluorescent detection: Why bother stripping and reprobing? Maximize your time and sample, and get the information you need in one shot, with multiplexing.
  2. Chemiluminescent detection: Working with low abundance targets or precious samples? Chemiluminescent detection gives you picogram-level sensitivity, letting you maximize the data you get from your sample.
  3. Protein normalization: Jess gives you an easy way to see if your samples contain a consistent protein load—just load her in-capillary protein normalization reagent into her assay plate and she'll take care of the rest. Her proprietary fluorescent reagent measures proteins immobilized in the same capillary as your immunoassay. The result? You can quickly see if your samples contain a consistent protein load, identify experimental setup and user errors, effectively normalize expression of your target protein to get accurate and consistent data, giving you the confidence you need in your results. Best of all, Jess's fluorescent detection capabilities enable two-color protein detection for multiplexing on top of protein normalization.
  4. Blot imaging: Still doing traditional Westerns? Snap! Get the picture with Jess's in-built blot imaging system.

Simple Western immunoassays take place in a capillary. Your sample, separation matrix, stacking matrix, antibodies and reagents are loaded automatically from a specially designed plate. Jess begins by aspirating the separation matrix and then the stacking matrix into each capillary. Next your sample is loaded, and capillaries are lowered to make contact with running buffer. Voltage is applied to enable separation by molecular weight. Once the separation is complete, UV light immobilizes the proteins to the capillary wall. With proteins now immobilized and the matrix cleared of the capillary, Jess starts the immunoprobing process, first with incubation with the primary antibody, followed by a secondary HRP conjugate, and finally chemiluminescent substrate. The chemiluminescent reaction is recorded by a CCD camera in a series of images over time. In just 3 hours you'll have quantitative, size-based data ready for analysis.

Her fluorescent detection capabilities enable two-color protein detection for multiplexing. During the immunoprobing process samples are incubated with the primary antibody, followed by infrared or near-infrared fluorescent secondary-tagged antibodies. Excitation of the fluorphores releases photons and the emission spectra is detected by wavelength sensors and recorded by a CCD camera in a series of images over time. In just 3 hours you'll have multiplexed, quantitative, size-based data ready for analysis.

Protein normalization has never been easier with Jess—just load her Protein Normalization Reagent into a row of wells on the plate, and she'll take care of the rest. The fluorescent-labeled reagent reacts with amines on proteins, enabling a between capillary comparison of protein load. Best of all, Jess's fluorescent detection capabilities enable two-color protein detection for multiplexing on top of protein normalization. Now, you can effectively normalize protein data, produce accurate and consistent data, and mitigate experimental setup and user error.

What does the data look like? At the end of your run, use the lane view option to compare band intensity or dive deep for fully quantitative analysis of protein size and concentration. Dive deeper into quantitative analysis to compare protein expression changes and analyze protein isoforms or size changes. Want to analyze expression changes between samples or compare runs? Our protein normalization will give you the confidence you need in your analysis.

Specifications
DESCRIPTION TOTAL PROTEIN
SPECIFICATION
CHEMILUMINESCENCE
SPECIFICATION
FLUORESCENCE
SPECIFICATION
PROTEIN NORMALIZATION
SPECIFICATION
Sample Required 0.3-1.2 µg 0.6-1.2 µg 2-4 µg 0.6-4 µg
Volume Required 3 µL/well
Size Range Molecular weight (MW) ladder ranges from 2-440 kDa
Sizing CV <10%
Intra-assay CV <15%
Inter-assay CV <20%
Resolution (± percent difference in MW) ± 15-20% for MW <20 kDA
± 10% for MW >20 kDa
Quantitation CV <20% N/A
Dynamic Range 2-3 logs 3-4 logs 3-4 logs 2-3 logs
Sensitivity ng Low pg High pg ng
Capillary 5 cm, 100 µm, 400 nL
Run time <3 hours <4 hours with immunoassay
Samples per run 13 or 25
Weight 23 kg
Dimensions (closed) 0.36 m H X 0.3 m W X 0.57 m D
Dimensions (open) 0.36 m H x 0.53 m W x 0.57 m D
Power US/CAN 120 V AC, 60 hz, 4.2 amps
Europe 240 AC, 50 Hz, 2.1 amps
Japan 100 AC, 50/60 Hz, 5.0 amps
Operating temperature 18-24 °C
Operating humidity 20-60% relative, non-condensing