Structure of ATP citrate lyase and the origin of citrate synthase in the Krebs cycle.

Verschueren KHG, Blanchet C, Felix J, Dansercoer A, De Vos D, Bloch Y, Van Beeumen J, Svergun D, Gutsche I, Savvides SN, Verstraete K, Nature 568(7753):571-575 (2019) Europe PMC

SASDE66 – C. limicola ATP-citrate lyase (ACL) in HBS

ATP-citrate lyase

MW^experimental	420	kDa
MW^expected	429	kDa
V^Porod	666	nm³

log I(s) 1.26×10⁵ 1.26×10⁴ 1.26×10³ 1.26×10²

ATP-citrate lyase small angle scattering data

s, nm^-1

Log plot Log-Log plot

ln I(s)

ln 1.27×10⁵ R_g: 6.1 nm 0 (6.1 nm)^-2 s²

(sR_g)²I(s)/I(0)

1.104 0 √3 sR_g

p(r)	R_g: 6.3 nm 0 D_max: 20 nm

Data validation

Experimental data range

p(r) fit to data

Metric

Value

s_min D_max / π

0.3

N_Shannon

Worse

Better

Metric

Value

p_cormap

χ²

0
4.713

Worse

Better

There are no models related to this curve.

Synchrotron SAXS data from solutions of C. limicola acetyl citrate lyase (ACL) in 20mM HEPES, 150mM NaCl, pH 7.2 were collected on the EMBL P12 beam line at the PETRA III storage ring (Hamburg, Germany) using a Pilatus 6M detector at a sample-detector distance of 3.1 m and at a wavelength of λ = 0.124 nm (l(s) vs s, where s = 4πsinθ/λ, and 2θ is the scattering angle). Size-exclusion chromatography SAXS (SEC-SAXS) was employed using a sample injection concentration of 17.50 mg/ml. Data were measured at through the SEC elution at 20°C. 900 successive 1 second frames were collected. The data were normalized to the intensity of the transmitted beam and radially averaged; the scattering of an appropriate solvent-blank was subtracted using the CHROMIXS SEC-SAXS analysis package.

SEC column = UNKNOWN. Sample injection volume = UNKNOWN. Flow rate = UNKNOWN

ATP-citrate lyase (ACL)
Mol. type		Protein
Organism		Chlorobium limicola
Olig. state		Tetramer
Mon. MW		107.3 kDa
Sequence		FASTA