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  • AlphaLISA Human and Mouse Mutant HTT Detection Kit, 5,000 Assay Points

AlphaLISA Human and Mouse Mutant HTT Detection Kit, 5,000 Assay Points

AlphaLISA Sandwich Anti-analyte Conjugated Acceptor Bead image
AlphaLISA Human and Mouse Mutant HTT Detection Kit, 5,000 Assay Points
AlphaLISA Sandwich Anti-analyte Conjugated Acceptor Bead image
AlphaLISA Sandwich Anti-analyte Conjugated Acceptor Bead

The AlphaLISA™ Mutant HTT kit is designed for the simple and rapid quantification of soluble HTT mutant proteins in cell lysate or brain tissues, providing results in a simplified, no-wash assay format compared to ELISA or western blot.

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Feature Specification
Application タンパク質定量
Protocol Time 3.5h at RT
Sample Volume 5 µL

The AlphaLISA™ Mutant HTT kit is designed for the simple and rapid quantification of soluble HTT mutant proteins in cell lysate or brain tissues, providing results in a simplified, no-wash assay format compared to ELISA or western blot.

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Unit Size: 100 assay points
Part #:
AL3205HV
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Unit Size: 500 assay points
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AL3205C
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Unit Size: 5,000 assay points
Part #:
AL3205F
For research use only. Not for use in diagnostic procedures. All products to be used in accordance with applicable laws and regulations including without limitation, consumption, and disposal requirements under European REACH regulations (EC 1907/2006).
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AlphaLISA Sandwich Anti-analyte Conjugated Acceptor Bead image
AlphaLISA Human and Mouse Mutant HTT Detection Kit, 5,000 Assay Points
AlphaLISA Sandwich Anti-analyte Conjugated Acceptor Bead image
AlphaLISA Sandwich Anti-analyte Conjugated Acceptor Bead

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Product information

  • Overview
  • How it works
  • Assay details
  • Assay validation
  • Specifications

Overview

Huntingtin (HTT) is a cytoplasmic protein which is highly expressed in the brain, and whose anti-apoptotic role is critical for neuronal survival. The wild-type (WT) protein has a functional structure, with a "normal" polyglutamine (polyQ) domain containing less than 36Q. The mutant HTT protein harbors an abnormally long polyQ tract (> 36Q) which causes the aggregation of the no longer functional protein. HTT aggregation leads to the selective neuronal cell death responsible for Huntington's Disease.

Formats

  • Our 100 assay point kit allows you to run 100 wells in 96-well format, using a 100 µL reaction volume (10 µL of sample).
  • Our 500 assay point kit allows you to run 500 wells in 96-well or 384-well format, using a 50 µL reaction volume (5 µL of sample).
  • Our 5,000 assay point kit allows you to run 5,000 wells in 96-well or 384-well format, using a 50 µL reaction volume (5 µL of sample

Features

  • No-wash steps, no separation steps
  • ELISA alternative technology
  • Sensitive detection
  • Broad sample compatibility
  • Small sample volume
  • Results in less than 4 hours

AlphaLISA technology allows the detection of molecules of interest in a no-wash, highly sensitive, quantitative assay. In an AlphaLISA assay, a biotinylated anti-analyte antibody binds to the Streptavidin-coated Donor beads while another anti-analyte antibody is conjugated to AlphaLISA Acceptor beads. In the presence of the analyte, the beads come into close proximity. The excitation of the Donor beads causes the release of singlet oxygen molecules that triggers a cascade of energy transfer in the Acceptor beads, resulting in a sharp peak of light emission at 615 nm.

How it works

Principle of the AlphaLISA Human & Mouse Mutant HTT assay

The AlphaLISA Mutant HTT assay is based on an AlphaLISA sandwich immunoassay involving a biotinylated anti-target antibody bound to Streptavidin-coated AlphaLISA Donor beads and an anti-target antibody conjugated to AlphaLISA Acceptor beads. One antibody is directed against the total HTT protein, and the second recognizes specifically the mutant polyQ domain. In the presence of the target, both antibodies bind to Mutant HTT, and the beads come into proximity. The excitation of the Donor beads provokes the release of singlet oxygen molecules that triggers a cascade of energy transfer within the Acceptor beads, resulting in emission with λmax at 615 nm. The intensity of the signal is directly proportional to the concentration of Mutant HTT present in the sample (cell lysate or tissue lysate).

Human & Mouse Mutant HTT Assay Principle

Protocol of the AlphaLISA human & mouse Mutant HTT assay

The AlphaLISA Mutant HTT assay can be run in a 96- or 384-well detection plate (50 µL final). As described here, samples (cell lysates or tissue lysates) or control lysate are dispensed directly into the assay plate for the detection of Mutant HTT by AlphaLISA reagents. No washing steps are needed. The protocol can be further miniaturized or upscaled by simply resizing each addition volume proportionally.

Protocol of the AlphaLISA human CCL17 assay

Assay details

Human & mouse mutant HTT assay details

Final assay volume 50 µL
Time to result 3.5 hours at RT
Kit component Lyophilized control lysate, SA-Donor Beads, Biotinylated anti-HTT, Anti-PolyQ conjugated Acceptor Beads, Assay Buffer, Lysis Buffer
Species Human & Mouse

Assay validation

Validation of AlphaLISA Mutant HTT detection kit on HEK293 transfected with different HTT plasmids

Four HTT plasmids were designed with different repeats of glutamine: 23, 48, 73 or 103 repeats were included in the protein sequence.

HEK293 cells were seeded in a 96-well culture-treated plate (25,000 cells/well) in complete culture medium, and incubated overnight at 37°C, 5% CO2. The cells were transfected with HTT plasmids. After 48h of incubation, the cells were lysed with 50 µL of AlphaLISA Lysis buffer (1X) supplemented with protease inhibitors for 30 minutes at RT under gentle shaking. 5 µL of each condition were transferred into a 384-well microplate before the sequential addition of AlphaLISA Total HTT and Mutant HTT detection reagents.

As expected, no signal was obtained with samples containing wild-type HTT (<36Q) either non transfected or Q23. The assay is therefore specific for mutant HTT (polyQ tail > 36Q) and the longer the expansion of the polyQ tail, the higher the signal will be even if the total concentration of protein was similar. The level of Total HTT protein remained constant for all the transfected plasmids tested.

Validation of Mutant HTT Detection Kit on HEK293 transfected cells

 

Validation on brain tissue samples collected from WT and mutant HTT mouse models

Briefly, a 10% (w/v) brain stem tissue homogenate was prepared using ice-cold 1X AlphaLISA Lysis Buffer (#AL003C) supplemented with protease inhibitors, and the insoluble fraction of the lysate containing putative mutant HTT aggregates was removed by centrifugation at 3500xg for 10 minutes at 4°C, and the supernatants containing soluble mutant HTT were collected for either direct analysis or dispensed into aliquots for storage at ≤-60°C.

The supernatants containing soluble HTT proteins were analyzed using the AlphaLISA Human & Mouse Total HTT Detection Kit and the AlphaLISA Human & Mouse Mutant HTT Detection Kit. To ensure that the detected analyte was assessed at a concentration compatible with the assay’s linear range, the lysates were pre-diluted just before detection in AlphaLISA Lysis Buffer supplemented with protease inhibitors just before detection (1/8 for Total HTT and Mutant assays).

As expected, no signal was obtained with the Mutant HTT assay on samples collected from WT mice, whereas the soluble mutant protein was clearly detected in tissue collected from premanifest zQ175 mice. Finally, the soluble total HTT protein (WT and mutant forms) was measured in all lysates at a similar level in both samples.

Analysis of brain tissue samples collected from WT and mutant HTT mouse models

Specifications

Application
Protein Quantification
Automation Compatible
Yes
Brand
AlphaLISA
Detection Modality
Alpha
Product Group
Kit
Protocol Time
3.5h at RT
Sample Volume
5 µL
Shipping Conditions
Shipped in Blue Ice
Target
HTT
Target Class
Biomarkers
Target Species
Human
Mouse
Technology
Alpha
Therapeutic Area
Neuroscience
Unit Size
5,000 assay points

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