Caged compounds for multichromic optical interrogation of neural systems

Amatrudo, Joseph M.; Olson, Jeremy P.; Agarwal, Hitesh K.; Ellis‐Davies, Graham C. R.

doi:10.1111/ejn.12785

Cited by 55 publications

(74 citation statements)

References 120 publications

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“…Subsequently several chromophores have been used for uncaging of biological signaling molecules with blue light 16–21 . Photochemical protecting groups sensitive to green light have also been reported 22–24 , but to our knowledge no biological studies have appeared with these probes.…”

Section: Introductionmentioning

confidence: 99%

Calcium Uncaging with Visible Light

et al. 2016

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We have designed a nitroaromatic photochemical protecting group that absorbs visible light in the violet-blue range. The chromophore is a dinitro derivative of bisstyrylthiophene (or BIST) that absorbs light very effectively (ε440 = 66,000 M−1 cm−1 and two-photon cross section of 350 GM at 775 nm). We developed a “caged calcium” molecule by conjugation of BIST to a Ca2+ chelator that upon laser flash photolysis rapidly releases Ca2+ in less than 0.2 ms. Using the patch-clamp method the optical probe, loaded with Ca2+, was delivered into acutely isolated mouse cardiac myocytes, where either one- and two-photon uncaging of Ca2+ induced highly local or cell-wide physiological Ca2+ signaling events.

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Section: Introductionmentioning

confidence: 99%

Calcium Uncaging with Visible Light

et al. 2016

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“…Since we have shown that DEAC450 uncaging is highly wavelength-selective for 2P excitation at 900 nm [27] , our data suggest the cloaked caged neurotransmitter G5-DEAC450-GABA could be very useful for chromatically selective, two-color optoneurobiology.…”

Section: Author Manuscript Author Manuscriptmentioning

confidence: 75%

“…Prior irradiation of the apical dendrite with 900nm (3 × 3 ms, 50 mW) elicited pronounced hyperpolarization, which blocked the action potential, which was restored when only short wavelength irradiation was used ( Figure 5). Since we have shown that DEAC450 uncaging is highly wavelength-selective for 2P excitation at 900 nm [27] , our data suggest the cloaked caged neurotransmitter G5-DEAC450-GABA could be very useful for chromatically selective, two-color optoneurobiology.Certainly it is the first example of a caged GABA compound that is highly active to 2P …”

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confidence: 75%

Cloaked Caged Compounds: Chemical Probes for Two‐Photon Optoneurobiology

et al. 2016

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Caged neurotransmitters, in combination with focused light beams, enable precise interrogation of neuronal function, even at the level of single synapses. However, most caged transmitters are, surprisingly, severe antagonists of ionotropic gamma-aminobutyric acid (GABA) receptors. By conjugation of a large, neutral dendrimer to a caged GABA probe we introduce a "cloaking" technology that effectively reduces such antagonism to very low levels. Such cloaked caged compounds will enable the study of the signaling of the inhibitory neurotransmitter GABA in its natural state using two-photon uncaging microscopy for the first time. Graphical abstractCaged neurotransmitters are known to be quite antagonistic toward the GABA-A receptor. The conjugation of a polyester dendrimer "cloak" to the caged compound DEAC450-GABA significantly decreased its GABA-A receptor antagonism. The chemical probe was inert at concentrations required for effective two-photon photolysis on living cells. Keywords caged compounds; GABA-A receptors; optical methods; two-photon; biologically inert Correspondence to: Graham C. R. Ellis-Davies. b These authors contributed equally to this work.Supporting information for this article is given via a link at the end of the document. HHS Public Access Author Manuscript Author ManuscriptAuthor Manuscript Author ManuscriptPhotochemical probes have revolutionized modern physiological studies. In an era initiated by Galvani, electrodes were the best technology available for real-time stimulation and measurement. However, the photon is more precise and versatile than the electron, so the former is not merely starting to "replace" the latter, but light, in combination with chemistry, is being used to open completely new avenues of physiological discovery [1] . To deliver their potential, the new chemical technologies require novel light sources and so pulsed lasers have been vital for time-resolved chemical biology [2] . Enabled by ultra-fast, pseudocontinuous Ti:sapphire lasers, neurobiology now routinely uses two-photon (2P) microscopy for live cell imaging in complex tissue such as acutely isolated brain slices and living animals. But, as noted by Denk, et al. in their seminal 1990 paper [3] , 2P excitation "also provides unprecedented capabilities for three-dimensional, spatially resolved photochemistry, particularly photolytic release of caged effector molecules." While initial reports of two-photon uncaging used probes [4,5] originally designed for linear actuation, more recently caged compounds designed for 2P excitation have been introduced for Glu, GABA, IP 3 , calcium, etc [6] . Some of these have even proved useful for independent 2P physiological studies [2] . It is striking that caged Glu probes, in particular, have proved very useful but caged GABA probes much less so. One reason for this must the inherent antagonism of all caged GABA compounds towards GABA-A receptors at concentrations required for effective 2P photolysis in brain tissue [7] . We have developed a new technology, which ...

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“…The γ-thiophosphate group impedes (Malmsjö et al, 2003), but does not completely prevent its enzymatic hydrolysis. A caged form of ATP 69 , which regenerates ATP upon irradiation has been studied and is potentially useful for studies of P2Rs (Amatrudo et al ., 2015). Similarly, the 1-(3,4-dimethyloxy-6-nitro-phenyl)ethyl (DMNPE) group was used to block the β-phosphate of agonist 65 to abolish its activity at the P2Y 1 R and P2Y 12 R, and this activity could be recovered upon irradiation (Gao et al ., 2008).…”

Section: P2yr Modulatorsmentioning

confidence: 99%

Medicinal chemistry of adenosine, P2Y and P2X receptors

2016

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Pharmacological tool compounds are now available to define action at the adenosine (ARs), P2Y and P2X receptors. We present a selection of the most commonly used agents to study purines in the nervous system. Some of these compounds, including A1 and A3 AR agonists, P2Y1R and P2Y12R antagonists, and P2X3, P2X4 and P2X7 antagonists, are potentially of clinical use in treatment of disorders of the nervous system, such as chronic pain, neurodegeneration and brain injury. Agonists of the A2AAR and P2Y2R are already used clinically, P2Y12R antagonists are widely used antithrombotics and an antagonist of the A2AAR is approved in Japan for treating Parkinson’s disease. The selectivity defined for some of the previously introduced compounds has been revised with updated pharmacological characterization, for example, various AR agonists and antagonists were deemed A1AR or A3AR selective based on human data, but species differences indicated a reduction in selectivity ratios in other species. Also, many of the P2R ligands still lack bioavailability due to charged groups or hydrolytic (either enzymatic or chemical) instability. X-ray crystallographic structures of AR and P2YRs have shifted the mode of ligand discovery to structure-based approaches rather than previous empirical approaches. The X-ray structures can be utilized either for in silico screening of chemically diverse libraries for the discovery of novel ligands or for enhancement of the properties of known ligands by chemical modification. Although X-ray structures of the zebrafish P2X4R have been reported, there is scant structural information about ligand recognition in these trimeric ion channels. In summary, there are definitive, selective agonists and antagonists for all of the ARs and some of the P2YRs; while the pharmacochemistry of P2XRs is still in nascent stages. The therapeutic potential of selectively modulating these receptors is continuing to gain interest in such fields as cancer, inflammation, pain, diabetes, ischemic protection and many other conditions. Reported potencies refer to the human receptors unless otherwise noted. Additional affinity data can be found in recent review papers (Müller and Jacobson, 2011; Jacobson et al., 2015; Coddou et al., 2011a).

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Caged compounds for multichromic optical interrogation of neural systems

Cited by 55 publications

References 120 publications

Calcium Uncaging with Visible Light

Calcium Uncaging with Visible Light

Cloaked Caged Compounds: Chemical Probes for Two‐Photon Optoneurobiology

Medicinal chemistry of adenosine, P2Y and P2X receptors

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