Mechanotransduction and the crayfish stretch receptor.

Mechanotransduction or mechanosensitivity is found in almost every cell in all organisms from bacteria to vertebrates. Mechanosensitivity covers a wide spectrum of functions from osmosensing, cell attachment, classical sensory mechanisms like tactile senses in the skin, detection of sound in hair cells of the hearing apparatus, proprioceptive functions like recording of muscle length and tension in the muscle spindle and tendon organ, respectively, and pressure detection in the circulation etc. Since most development regarding the molecular aspects of the mechanosensitive channel has been made in nonsensory systems it is important to focus on mechanosensitivity of sensory organs where the functional importance is undisputed. The stretch receptor organ of the crustaceans is a suitable preparation for such studies. The receptor organ is experimentally accessible to mechanical manipulation and electrophysiological recordings from the sensory neuron using intracellular microelectrode or patch clamp techniques. It is also relatively easy to inject substances into the neuron, which also makes the neuron accessible to measurements with fluorescent techniques. The aim of the present paper is to give an up to date summary of observations made on the transducer properties of the crayfish stretch receptor (Astacus astacus and Pacifastacus leniusculus) including some recent unpublished findings. Finally some aspects on future line of research will be presented.

Ion channels for mechanotransduction in the crayfish stretch receptor.

Mechanosensitivity is found in almost every cell in all organisms from bacteria to vertebrates and covers a wide spectrum of function from osmosensing to mechanical sensing in the specialized receptors, such as the hair cells of the cochlea. The molecular substrate for such mechanosensitivity is thought to be mechanosensitive ion channels (MSCs). Because most development regarding the molecular aspects of the MSC has been made in nonsensory or sensory systems, which have not been accessible to recordings from ion channels, it is important to focus on the mechanosensitivity of sensory organs where their functional importance is undisputed. The stretch receptor organ (SRO) of the crustaceans is a suitable preparation for such studies. Each organ contains two receptors: one slowly and one rapidly adapting receptor neurons. The primary mechanosensitivity is generated by two types of MSC of hitherto unknown molecular type located in the neuronal dendrites, which are inserted into a receptor muscle fiber. In addition to the MSCs, the neurons contain voltage-gated Na(+) channels, which seem to be differently located in the slowly and rapidly adapting neurons. At least three types of voltage-gated K(+) channels are present in the sensory neurons, the location of which is not known. The spatial distribution of ion channels and the kinetics of the channels, together with the viscoelastic properties of the receptor muscles, determine the overall transducer properties and impulse firing of the two receptor neurons, including their typical adaptive characteristics.

An M-like potassium current in the guinea pig cochlea.

Potassium M currents play a role in stabilizing the resting membrane potential. These currents have previously been identified in several cell types, including sensory receptors. Given that maintaining membrane excitability is important for mechano-electrical transduction in the inner ear, the presence of M currents was investigated in outer hair cells isolated from the guinea pig hearing organ. Using a pulse protocol designed to emphasize M currents with the whole-cell patch-clamp technique, voltage- and time-dependent, non-inactivating, low-threshold currents (the hallmarks of M currents) were recorded. These currents were significantly reduced by cadmium chloride. Results from RT-PCR analysis indicated that genes encoding M channel subunits KCNQ2 and KCNQ3 are expressed in the guinea pig cochlea. Our data suggest that guinea pig outer hair cells express an M-like potassium current that, following sound stimulation, may play an important role in returning the membrane potential to resting level and thus regulating outer hair cell synaptic mechanisms.

The low conductance K(+) channel in human colonic crypt cells has a voltage-dependent permeability not affected by Mg(++).

The low conductance K(+) channel found in human colonocytes was investigated using the patch-clamp technique. The channel is Ca(++)-dependent and is blocked by Ba(++) (5 mM) with a decrease in open probability from 0.42 to 0.19. At -40 mV the slope conductance was 29 pS (using intracellular solution in the pipette). In inside-out patches, inward rectification was seen both with KCl (pipette)/NaCl (bath) solutions as well as KCl/KCl solutions. The rectification could not be affected by omitting Mg(++) from the pipette or the bath solution, neither by exposing the patches to the polyamine spermine (1 mM). Using the Goldman-Hodgkin-Katz equation we show that the permeability decreased in a linear fashion from approximately 5.2 x 10(-14) cm(3)/s to 1.8 x 10(-14) cm(3)/s (-100 to +100 mV), both with and without Mg(++) in the solutions. There was no significant difference in the nominal values of permeability. This property of the K(+) channel may facilitate the hyperpolarization needed to sustain a chloride secretion.