SUIT-020: Difference between revisions

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SUIT-020

Description

File:SUIT-020 O2 mt D032.png

Reference: A: »Versions

MitoPedia concepts: MiP concept, SUIT protocol, SUIT A, Recommended

MitoPedia methods: Respirometry, Fluorometry

SUIT-category:

SUIT protocol pattern:

DLP applications

SUIT-020 Fluo mt D033 simultaneous determination of O₂ flux and mt-membrane potential using any fluorescence dye (Safranin, TMRM etc) on isolated mitochondria and tissue homogenate.
SUIT-020 Fluo mt D036 simultaneous determination of O₂ flux and mt-membrane potential using any fluorescence dye (Safranin, TMRM etc) on isolated mitochondria and tissue homogenate.

SUIT-020 O2 mt D032 determination of O₂ flux on isolated mitochondria and tissue homogenate as a control for SUIT-020 Safr mt D033.
SUIT-020 O2 mt D035 determination of O₂ flux on isolated mitochondria and tissue homogenate as a control for SUIT-020 Safr mt D036.

References

	Year	Reference	Organism	Tissue;cell
MiPNet20.13 Safranin mt-membranepotential	2019-06-24	O2k-FluoRespirometry: HRR and simultaneous determination of mt-membrane potential with safranin or TMRM.	Mouse	Nervous system
Krumschnabel 2014 Methods Enzymol	2014	Krumschnabel G, Eigentler A, Fasching M, Gnaiger E (2014) Use of safranin for the assessment of mitochondrial membrane potential by high-resolution respirometry and fluorometry. Methods Enzymol 542:163-81. https://doi.org/10.1016/B978-0-12-416618-9.00009-1	Mouse	Nervous system

Steps and respiratory states

Step	State	Pathway	Q-junction	Comment - Events (E) and Marks (M)
1PM	PM_L(n)	N	CI	1PM NADH-linked substrates (type N-pathway to Q). Non-phosphorylating resting state (LEAK state); LEAK respiration L(n) in the absence of ADP, ATP, AMP (no adenylates).
2D	PM_P	N	CI	1PM;2D NADH-linked substrates (type N-pathway to Q). OXPHOS capacity P (with saturating [ADP]), active OXPHOS state.
2c	PMc_P	N	CI	1PM;2D;2c NADH-linked substrates (type N-pathway to Q). Addition of cytochrome c yields a test for integrity of the mtOM (cytochrome c control efficiency). Stimulation by added cytochrome c would indicate an injury of the mtOM and limitation of respiration in the preceding state without added c due to loss of cytochrome c. Typically, cytochrome c is added immediately after the earliest ADP-activation step (OXPHOS capacity P with saturating [ADP]). OXPHOS capacity P (with saturating [ADP]), active OXPHOS state.
3G	PGM_P	N	CI	1PM;2D;2c;3G NADH-linked substrates (type N-pathway to Q). OXPHOS capacity P (with saturating [ADP]), active OXPHOS state.
4S	PGMS_P	NS	CI&II	1PM;2D;2c;3G;4S Respiratory stimulation by simultaneous action of type N substrates & succinate, with convergent electron flow in the NS-pathway for reconstitution of TCA cycle function. OXPHOS capacity P (with saturating [ADP]), active OXPHOS state.
5Rot	S_P	S	CII	1PM;2D;2c;3G;4S;5Rot Succinate, S ( type S-pathway to Q). Succinate pathway control state (S-pathway) after inhibiting CI with rotenone, which also inhibits the F-pathway.
6Omy	S_L(Omy)			1PM;2D;2c;3G;4S;5Rot;6Omy Non-phosphorylating resting state (LEAK state); LEAK-respiration, L(Omy), after blocking the ATP synthase with oligomycin.
7U*	S_E	S	CII	1PM;2D;2c;3G;4S;5Rot;6Omy;7S Succinate, S ( type S-pathway to Q). Uncoupler titration (avoiding inhibition by high uncoupler concentrations) to obtain electron transfer (ET) capacity E (noncoupled ET-state). Test for limitation of OXPHOS capacity P by the phosphorylation system (ANT, ATP synthase, phosphate transporter) relative to ET capacity E in mt-preparations: E-P control efficiency and E-L coupling efficiency. In living cells: E-R control efficiency and E-L coupling efficiency. Noncoupled electron transfer state, ET state, with ET capacity E.
8Ama	ROX			1PM;2D;2c;3G;4S;5Rot;6Omy;7S;8Ama Rox is the residual oxygen consumption in the ROX state, due to oxidative side reactions, estimated after addition of antimycin A (inhibitor of CIII). Rox is subtracted from oxygen flux as a baseline for all respiratory states, to obtain mitochondrial respiration (mt).

Step	Respiratory state	Pathway control	ET-Complex	Comment
## AsTm	AsTm_E	CIV	CIV
## Azd	CHB

Bioblast links: SUIT protocols - >>>>>>> - Click on [Expand] or [Collapse] - >>>>>>>

Coupling control

» Coupling control state

» ET capacity

» OXPHOS capacity

» LEAK respiration

Pathway control

» Electron transfer pathway

» Fatty acid oxidation pathway control state, F

» NADH electron transfer-pathway state, N

» Succinate pathway control state, S

» NS-pathway control state, NS

» Glycerophosphate pathway control state, Gp

» Complex IV single step, CIV

» Anaplerotic pathway control state

Main fuel substrates

» Glutamate, G

» Glycerophosphate, Gp

» Malate, M

» Octanoylcarnitine, Oct

» Pyruvate, P

» Succinate, S

Glossary

» List of SUIT states

» SUIT concept

Strengths and limitations

+ Information in one protocol about the NS, S and N-pathway control state.

- The fluorescence dye (such as Safranin, TMRM etc) can inhibit most porbably the NADH-linked respiration, therefore, the protocol has to be run without using the fluorescence dye. The following protocols can be used: SUIT-020 O2 mt D032, SUIT-020 O2 mt D035.

Compare SUIT protocols

SUIT-001

@@ Line 16: / Line 16: @@
 == DLP applications ==
-:::* [[SUIT-020 Safr mt D033]]  simultaneous determination of O<sub>2</sub> flux and mt-membrane potential using [[Safranin]] on isolated mitochondria and tissue homogenate.
+:::* [[SUIT-020 Fluo mt D033]]  simultaneous determination of O<sub>2</sub> flux and mt-membrane potential using any fluorescence dye ([[Safranin]], [[TMRM]] etc) on isolated mitochondria and tissue homogenate.
-:::* [[SUIT-020 Safr mt D036]] simultaneous determination of O<sub>2</sub> flux and mt-membrane potential using [[Safranin]] on isolated mitochondria and tissue homogenate.
+:::* [[SUIT-020 Fluo mt D036]]  simultaneous determination of O<sub>2</sub> flux and mt-membrane potential using any fluorescence dye ([[Safranin]], [[TMRM]] etc) on isolated mitochondria and tissue homogenate.
-:::* [[SUIT-020 TMRM mt D034]] simultaneous determination of O<sub>2</sub> flux and mt-membrane potential using [[TMRM]] on isolated mitochondria and tissue homogenate.
+:::* [[SUIT-020 O2 mt D032]] determination of O<sub>2</sub> flux on isolated mitochondria and tissue homogenate as a control for SUIT-020 Safr mt D033.
-:::* [[SUIT-020 TMRM mt D037]] simultaneous determination of O<sub>2</sub> flux and mt-membrane potential using [[TMRM]] on isolated mitochondria and tissue homogenate.
+:::* [[SUIT-020 O2 mt D035]] determination of O<sub>2</sub> flux on isolated mitochondria and tissue homogenate as a control for SUIT-020 Safr mt D036.
-:::* [[SUIT-020 O2 mt D032]] determination of O<sub>2</sub> flux on isolated mitochondria and tissue homogenate.
-:::* [[SUIT-020 O2 mt D035]] determination of O<sub>2</sub> flux on isolated mitochondria and tissue homogenate.
@@ Line 44: / Line 41: @@
 == Strengths and limitations ==
 :::+ Information in one protocol about the NS, S and N-pathway control state.
-:::- The fluorescence dye (Safranin, TMRM) can inhibit most porbably the NADH-linked respiration, therefore, the protocol has to be run without using the fluorescence dye. The following protocols can be used: [[SUIT-020 O2 mt D032]], [[SUIT-020 O2 mt D035]].
+:::- The fluorescence dye (such as Safranin, TMRM etc) can inhibit most porbably the NADH-linked respiration, therefore, the protocol has to be run without using the fluorescence dye. The following protocols can be used: [[SUIT-020 O2 mt D032]], [[SUIT-020 O2 mt D035]].
 :::