Mn<sup>2+</sup>‐Phos‐Tag Polyacrylamide for the Quantification of Protein Phosphorylation Levels

Markandran, Kasturi; Xuan, Jane Vanetta Lee En; Yu, Hongwei; Shun, Lim Meng; Ferenczi, Michael A.

doi:10.1002/cpz1.221

Cited by 3 publications

(5 citation statements)

References 86 publications

(79 reference statements)

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“…40 μmol/L MnCl 2 and 20 μmol/L phos-tag (Wako #304-93521) were added to the SDS-PAGE (8 %). After the electrophoresis, the phos-tag gels were incubating with transfer buffer containing 5 mM EDTA for 20 minutes twice to remove the divalent cations 49 . Washing with transfer buffer for 10 minutes once.…”

Section: Methodsmentioning

confidence: 99%

α-synucleinopathy associated calcium overload and autophagy failure is regulated by gain-of-function of Tousled-like kinase

Gong

Chen

Xiong

et al. 2022

Preprint

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As a pathological hallmark in Parkinson’s disease (PD), α-synucleinopathy causes multiple cellular damages, including calcium overload, mitochondrial and autophagic dysfunction, and eventually dopamine neuron death. However, the hierarchy of these detrimental events is unclear. In Drosophila, we confirmed that overexpression of α-synuclein could induce all these cytotoxic events. To determine the specific cytotoxic events induced by calcium overload, we established a calcium overload model in Drosophila and performed genetic screens. We found that calcium overload caused mitochondrial damage and autophagy failure and cell death, and these cytotoxic processes could be strongly rescued by loss of Tousled-like kinase (TLK). Interestingly, loss of TLK also rescued defects induced by α-synuclein overexpression in Drosophila. This suggests that calcium overload acts as the crucial event upstream of mitochondrial and autophagy dysfunction. For TLK regulation of autophagy, our data indicated that a transcriptional factor REPTOR, which regulated the expression of several lysosomal genes, functioned downstream of TLK. In mammalian cells and mice, TLK2 (the homolog of Drosophila TLK) was phosphorylated under calcium overload. Upon phosphorylation, TLK2 increased its kinase activity. In addition, TLK2 could phosphorylate CREBRF (the human homolog of REPTOR) to cause its loss of transcription on the lysosomal genes. Moreover, TLK2 knockout mice rescued multi-aspect cytotoxicity induced by calcium overload and α-synuclein overexpression. Our research demonstrates that TLK2 acts as a key regulator to mediate cell death and dysfunctions of mitochondria and autophagy downstream of calcium overload.

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Section: Methodsmentioning

confidence: 99%

α-synucleinopathy associated calcium overload and autophagy failure is regulated by gain-of-function of Tousled-like kinase

Gong

Chen

Xiong

et al. 2022

Preprint

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“…The details of the antibodies used are presented in Table S6 . A comprehensive guide for using Phos-tag gels is provided in [ 104 ].

…”

Section: Methodsmentioning

confidence: 99%

“…The details of the antibodies used are presented in Table S6. A comprehensive guide for using Phos-tag gels is provided in [104]. The methodology used to quantify enzyme expression was exactly the same as described previously in Section 2.3.…”

Section: Measurement Of Sarcomeric Protein Phosphorylationmentioning

confidence: 99%

Functional and Molecular Characterisation of Heart Failure Progression in Mice and the Role of Myosin Regulatory Light Chains in the Recovery of Cardiac Muscle Function

Markandran

Song

et al. 2021

IJMS

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Heart failure (HF) as a result of myocardial infarction (MI) is a major cause of fatality worldwide. However, the cause of cardiac dysfunction succeeding MI has not been elucidated at a sarcomeric level. Thus, studying the alterations within the sarcomere is necessary to gain insights on the fundamental mechansims leading to HF and potentially uncover appropriate therapeutic targets. Since existing research portrays regulatory light chains (RLC) to be mediators of cardiac muscle contraction in both human and animal models, its role was further explored In this study, a detailed characterisation of the physiological changes (i.e., isometric force, calcium sensitivity and sarcomeric protein phosphorylation) was assessed in an MI mouse model, between 2D (2 days) and 28D post-MI, and the changes were related to the phosphorylation status of RLCs. MI mouse models were created via complete ligation of left anterior descending (LAD) coronary artery. Left ventricular (LV) papillary muscles were isolated and permeabilised for isometric force and Ca2+ sensitivity measurement, while the LV myocardium was used to assay sarcomeric proteins’ (RLC, troponin I (TnI) and myosin binding protein-C (MyBP-C)) phosphorylation levels and enzyme (myosin light chain kinase (MLCK), zipper interacting protein kinase (ZIPK) and myosin phosphatase target subunit 2 (MYPT2)) expression levels. Finally, the potential for improving the contractility of diseased cardiac papillary fibres via the enhancement of RLC phosphorylation levels was investigated by employing RLC exchange methods, in vitro. RLC phosphorylation and isometric force potentiation were enhanced in the compensatory phase and decreased in the decompensatory phase of HF failure progression, respectively. There was no significant time-lag between the changes in RLC phosphorylation and isometric force during HF progression, suggesting that changes in RLC phosphorylation immediately affect force generation. Additionally, the in vitro increase in RLC phosphorylation levels in 14D post-MI muscle segments (decompensatory stage) enhanced its force of isometric contraction, substantiating its potential in HF treatment. Longitudinal observation unveils potential mechanisms involving MyBP-C and key enzymes regulating RLC phosphorylation, such as MLCK and MYPT2 (subunit of MLCP), during HF progression. This study primarily demonstrates that RLC phosphorylation is a key sarcomeric protein modification modulating cardiac function. This substantiates the possibility of using RLCs and their associated enzymes to treat HF.

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“…The electrophoresis duration, Phos-tag concentration and protein amount to be loaded were systematically optimised to use the gel effectively. The systematic approach for optimisation is recorded in the manuscript published in Current Protocols (273).…”

Section: Phos-tag Gel Electrophoresis Proceduresmentioning

confidence: 99%

“…, where 0P, 1P and 2P refers to zero, singly and doubly phosphorylated protein bands, respectively. Although phos-tag gel electrophoresis and western blotting can be a tedious procedure requiring thorough optimisation, it is relatively cheap and produce a reasonable output of data per gel (273). Thus, this was chosen over other techniques such as ELISA and mass spectrometry (273).…”

Section: Rlc Phosphorylation =mentioning

confidence: 99%

Investigating the role of phosphorylated regulatory light chains during heart failure progression

Markandran¹

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Mn²⁺‐Phos‐Tag Polyacrylamide for the Quantification of Protein Phosphorylation Levels

Cited by 3 publications

References 86 publications

α-synucleinopathy associated calcium overload and autophagy failure is regulated by gain-of-function of Tousled-like kinase

α-synucleinopathy associated calcium overload and autophagy failure is regulated by gain-of-function of Tousled-like kinase

Functional and Molecular Characterisation of Heart Failure Progression in Mice and the Role of Myosin Regulatory Light Chains in the Recovery of Cardiac Muscle Function

Investigating the role of phosphorylated regulatory light chains during heart failure progression

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Mn2+‐Phos‐Tag Polyacrylamide for the Quantification of Protein Phosphorylation Levels

Cited by 3 publications

References 86 publications

α-synucleinopathy associated calcium overload and autophagy failure is regulated by gain-of-function of Tousled-like kinase

α-synucleinopathy associated calcium overload and autophagy failure is regulated by gain-of-function of Tousled-like kinase

Functional and Molecular Characterisation of Heart Failure Progression in Mice and the Role of Myosin Regulatory Light Chains in the Recovery of Cardiac Muscle Function

Investigating the role of phosphorylated regulatory light chains during heart failure progression

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Mn²⁺‐Phos‐Tag Polyacrylamide for the Quantification of Protein Phosphorylation Levels