Date published: 2025-9-11

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KV1.7 Activators

KV1.7 activators refer to a class of chemical compounds that selectively bind to and modulate the activity of the KV1.7 potassium channel, a type of voltage-gated potassium channel (VGKC). These channels are integral membrane proteins that facilitate the selective flow of potassium ions across the cell membrane, which is crucial for maintaining the membrane potential and regulating cellular excitability. KV1.7 channels, like other family members, consist of four subunits that come together to form a pore through which potassium ions can pass in response to changes in the electrical potential across the cell membrane. Activators of KV1.7 channels are distinguished by their ability to increase the channel's open-probability or shift its voltage-dependence of activation, thereby enhancing the potassium current through these channels under conditions where they would normally be less active or inactive.

The action of KV1.7 activators at the molecular level involves specific interactions with the channel protein that lead to alterations in its conformational state, promoting the opening of the channel pore. These interactions may stabilize the open state or destabilize the closed state of the channel, depending on the binding site and the nature of the activator. The chemical structures of KV1.7 activators are diverse, and their design is often informed by the detailed structural and functional characteristics of the KV1.7 channel. The chemical complexity of these activators is reflected in their specificity and selectivity for the KV1.7 channel, as they must discriminate this particular channel subtype from other closely related VGKCs. Effective activators typically exhibit a high affinity for KV1.7, ensuring that they can modulate the channel's activity at relatively low concentrations, and their binding is often reversible, allowing for a controlled modulation of channel activity. The development of these compounds involves sophisticated techniques in chemistry, computational modeling, and electrophysiological testing to fine-tune their interactions with the channel and to maximize their selectivity and potency.

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