Sodium nitroprusside alters dark voltage and light responses in isolated retinal rods during whole-cell recording

Schmidt, K.; Nöll, Gottfried N.; Yamamoto, Yoshihiko

doi:10.1017/s0952523800009664

Cited by 46 publications

(19 citation statements)

References 22 publications

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“…Since cGMP is formed in bation with 1 ktM nicardipine, or 1 p~M verapamil (data not mammalian cells by the guanylate cyclase catalysed hydrolysis shown). A possible explanation for the observed potentiation of GTP [21], the above procedure may have resulted in the in the cGMP-evoked increase in [CaZ+]i following Ca 2+ store inhibition of guanylate cyclase, and a corresponding decrease depletion is a decrease in cytoplasmic Ca 2+ buffering due to in the free cytoplasmic level of cGMP in the above studies. If inhibition of Ca 2+ uptake into stores by thapsigargin.…”

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confidence: 75%

Calcium store depletion potentiates a phosphodiesterase inhibitor‐ and dibutyryl cGMP‐evoked calcium influx in rat pituitary GH₃ cells

Willmott¹,

Asselin²,

Galione³

1996

FEBS Letters

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A role for cGMP in the control of capacitative Ca 2+ two [9]. Also, it has been suggested that the calcium-releaseinflux was identified in rat pituitary GH3 cells. Application of activated calcium (CRAC) channel, involved in capacitative 50 ~tM-1 mM of the non-specific phosphodiesterase inhibitor, Ca 2+ influx, might be analogous to the transient receptor 3-isobutyl-l-methylxanthine (IBMX), or the specific cGMPpotential (trp) gene product in Drosophila photoreceptors phosphodiesterase inhibitor, zaprinast, induced a dose-dependent [6], which has been shown to possess significant amino acid Preparation of cellsRat pituitary GH3 cells were seeded onto polylysine-coated borosi-1. Introduction licate glass cover-slips in 6-well plates, and were grown in Hams F10 medium supplemented with 16% foetal calf serum for 34 days. For Ca 2+ imaging experiments, cells were loaded with 2 ~tM fura-2 AM in The cyclic nucleotides, cGMP and cAMP, have long been 2 ml Hank's medium (pH 7.2) in the presence of 0.1% Pluronic for 45 established as important second messengers in a variety of cell min at room temperature. Cover slips were rinsed in Hank's medium signalling pathways [1,2]. Roles for these species in intraceland were then transferred to a teflon cover-slip holder and 900 p3 lular Ca 2+ signalling and homeostasis are also apparent. Most Hank's medium added. The cover-slip dish was placed on the stage of an inverted Zeiss Axiovert 35 microscope for Ca 2+ imaging. notably, cAMP stimulates Ca r+ influx through L-type Ca r+ channels of rat pancreatic [~-cells [3] Video ratio image analysis of GH3 cell [Ca2+]i was performed using an ion imaging system supplied by 'Improvision', Coventry, UK, in a channels [1], inhibits Ca r+ influx in other excitable cells by similar way as previously described [5]. Cells were loaded with the directly affecting voltage-gated Ca r+ channels [4], and moduacetoxymethyl (AM) ester of Fura-2 (Molecular Probes Inc.). Free lates Ca r+ influx in non-excitable cells [4]. In addition, cGMP cytosolic Ca 2+ concentration was determined by taking the ratio of has also been shown to stimulate the synthesis of the potent fluorescence intensities at excitation wavelengths 340 and 380 nm, Ca r+ mobilizing agent, cylic-ADP-ribose, in sea urchin eggs using an emission wavelength of 510 nm. Pairs of 340 and 380 nm images were captured every 3 s and ratio images were calculated using [5]. Although the above indicate specific roles for cyclic nu-

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confidence: 75%

Calcium store depletion potentiates a phosphodiesterase inhibitor‐ and dibutyryl cGMP‐evoked calcium influx in rat pituitary GH₃ cells

Willmott¹,

Asselin²,

Galione³

1996

FEBS Letters

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“…There is also evidence from recent studies that NO is involved in several different processes in the vertebrate retina, for example it influences light responses of amphibian rods [4,5], it activates a soluble guanylyl cyclase and modulates a Ca 2+ channel and a voltage-independent conductance in inner segments of photoreceptors [6,7]. Effects of NO were also recorded on hemi-gap junction channels in horizontal cells [8], on cGMP-gated cation channels in retinal ganglion [9] and on-bipolar cells [10].…”

Section: Introductionmentioning

confidence: 99%

Purified retinal nitric oxide synthase enhances ADP‐ribosylation of rod outer segment proteins

Zoche

Koch

1995

FEBS Letters

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Nitric oxide synthase is present in different cell layers of vertebrate retina and seems to have neuromodulatory functions in the outer retina. The enzyme, when purified from a bovine retina extract, has an apparent molecular mass of 160 kDa and resembles the neuronal constitutive NOS type I with respect to CaZ+-calmodulin sensitivity, K m value and inhibition by analogues of L-arginine. Retinal NOS is present in a preparation of rod outer segments attached to parts of the inner segments, but not in pure outer segments. We describe the enhancement of specific ADP-ribosylation of outer segment proteins by purified retinal NOS.

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“…This is supported by evidence that NADPH diaphorase is a NOS (8,9) as well as by evidence that NO plays a functional role in the outer retina. Involvement of NO in photoreceptor function is (15)(16)(17)(18), (ii) photoreceptor responses to light are modulated by NO relevant substances (e.g., NO releasing substance sodium nitroprusside, NADPH, arginine) (15), and (iii) NOS has been localized in salamander rod and cone ellipsoids by immunocytochemistry (23) and in bovine rod outer segments by enzymatic assay (17). Furthermore, other studies have suggested that NO may be involved in the process of photoreceptor adaptation (15).…”

Section: Discussionmentioning

confidence: 99%

“…Involvement of NO in photoreceptor function is (15)(16)(17)(18), (ii) photoreceptor responses to light are modulated by NO relevant substances (e.g., NO releasing substance sodium nitroprusside, NADPH, arginine) (15), and (iii) NOS has been localized in salamander rod and cone ellipsoids by immunocytochemistry (23) and in bovine rod outer segments by enzymatic assay (17). Furthermore, other studies have suggested that NO may be involved in the process of photoreceptor adaptation (15). The possibility that inner segment NADPH diaphorase labeling may result from the presence of an oxidative enzyme other than NOS has been raised by results in rat retina (24), although those results may simply reflect the involvement of a different NOS isoenzyme.…”

Section: Discussionmentioning

confidence: 99%

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Differentiation of short-wavelength-sensitive cones by NADPH diaphorase histochemistry.

Petry¹,

Murphy²

1995

Proc. Natl. Acad. Sci. U.S.A.

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In addition to providing the basis for color vision, the spectral classes of mammalian cone photoreceptors contribute differentially to other aspects of vision. Specifically, the shortwavelength-sensitive (SWS or "blue-sensitive") cone mechanism differs from other cone mechanisms by exhibiting poorer spatial acuity, low temporal resolution, response saturation at low light levels, longer response latencies, and lack of an off-response (1). The poor spatial acuity has been linked to the low density and unique distribution of SWS cone photoreceptors (2), but the other anomalous characteristics of the SWS cone mechanism usually are attributed to postreceptoral processes (1,3,4). Yet, SWS cones have also been shown to differ biochemically from other cones types. For example, S antigen (also known as 48-kDa protein and arrestin) is present in SWS cones (5), and carbonic anhydrase is absent in SWS cones (6). This study addresses another difference of SWS cones, the pattern of NADPH diaphorase (NADPH dehydrogenase; EC 1.6.99.1) histochemistry in their cellular subcompartments.NADPH diaphorase histochemistry is based on the NADPH-dependent conversion of a soluble tetrazolium salt to an insoluble, visible formazan (7). Neuronal NADPH diaphorase has been shown to be a nitric oxide synthase (NOS) (8, 9) and NADPH diaphorase histochemistry provides a robust method to describe the distribution of NOS in the brain (e.g., ref. 10). As a neural messenger, neuronal nitric oxide (NO) diffuses across cellular membranes to activate soluble guanylate cyclase, which in turn increases intracellular levels of second messenger cGMP (11). NO has been implicated in synaptic transmission and plasticity (12)(13)(14) and also in photoreceptor function (15-18). In the vertebrate retina, NADPHThe publication costs of this article were defrayed in part by page charge payment. This article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. §1734 solely to indicate this fact. (27). In no instance has differential staining of spectral classes of cones been reported.In contrast to these previous studies of rod-dominated mammalian retinae, we present work that was undertaken to study NADPH diaphorase histochemistry in a cone-dominated mammalian retina. The tree shrew (Tupaia) has long been of interest to neuroscientists because of its well-developed central visual system and its close taxonomic relationship to primates (28). We elected to study this species because 95% of tree shrew photoreceptors are cones (29) and only two spectral types are represented: SWS and long-wavelength-sensitive (LWS) cones (30,31). Furthermore, the triangular packing distribution and relative density of tree shrew SWS cones are representative of that observed in other mammals, including primates (29,31,32). In addition, the spectral sensitivity and deutan-type dichromatic color vision of this species have been well characterized by electroretinography and psychophysics (33)(34)(35). Thus, the tree shrew retina offers an excellent model to study...

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Sodium nitroprusside alters dark voltage and light responses in isolated retinal rods during whole-cell recording

Cited by 46 publications

References 22 publications

Calcium store depletion potentiates a phosphodiesterase inhibitor‐ and dibutyryl cGMP‐evoked calcium influx in rat pituitary GH₃ cells

Calcium store depletion potentiates a phosphodiesterase inhibitor‐ and dibutyryl cGMP‐evoked calcium influx in rat pituitary GH₃ cells

Purified retinal nitric oxide synthase enhances ADP‐ribosylation of rod outer segment proteins

Differentiation of short-wavelength-sensitive cones by NADPH diaphorase histochemistry.

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Sodium nitroprusside alters dark voltage and light responses in isolated retinal rods during whole-cell recording

Cited by 46 publications

References 22 publications

Calcium store depletion potentiates a phosphodiesterase inhibitor‐ and dibutyryl cGMP‐evoked calcium influx in rat pituitary GH3 cells

Calcium store depletion potentiates a phosphodiesterase inhibitor‐ and dibutyryl cGMP‐evoked calcium influx in rat pituitary GH3 cells

Purified retinal nitric oxide synthase enhances ADP‐ribosylation of rod outer segment proteins

Differentiation of short-wavelength-sensitive cones by NADPH diaphorase histochemistry.

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Calcium store depletion potentiates a phosphodiesterase inhibitor‐ and dibutyryl cGMP‐evoked calcium influx in rat pituitary GH₃ cells

Calcium store depletion potentiates a phosphodiesterase inhibitor‐ and dibutyryl cGMP‐evoked calcium influx in rat pituitary GH₃ cells