Structure and Function of Gli123 Involved in Mycoplasma mobile Gliding.

Matsuike D, Tahara YO, Nonaka T, Wu HN, Hamaguchi T, Kudo H, Hayashi Y, Arai M, Miyata M, J Bacteriol :e0034022 (2023) Europe PMC

SASDQ88 – recombinant p123 expressed protein (Gli123)

p123 expressed protein

MW^experimental	273	kDa
MW^expected	248	kDa
V^Porod	436	nm³

log I(s) 2.45×10^-2 2.45×10^-3 2.45×10^-4 2.45×10^-5

p123 expressed protein small angle scattering data

s, nm^-1

Log plot Log-Log plot

ln I(s)

ln 2.45×10^-2 R_g: 8.2 nm 0 (8.2 nm)^-2 s²

(sR_g)²I(s)/I(0)

1.104 0 √3 sR_g

p(r)	R_g: 9 nm 0 D_max: 31.6 nm

Data validation

Experimental data range

p(r) fit to data

Metric

Value

s_min D_max / π

0.8

N_Shannon

Worse

Better

Metric

Value

p_cormap

χ²

0.634
1.139

Worse

Better

Fits and models

log I(s)	s, nm^-1
+3 Δ/σ -3	s, nm^-1

Synchrotron SAXS data from solutions of recombinant Gli123 in 100 mM ammonium acetate, pH 6.8 were collected on the BL-10C beam line at the Photon Factory (PF), High Energy Accelerator Research Organization (KEK; Tsukuba, Japan) using a Pilatus3 2M detector at a sample-detector distance of 2.1 m and at a wavelength of λ = 0.1488 nm (I(s) vs s, where s = 4πsinθ/λ, and 2θ is the scattering angle). In-line size-exclusion chromatography (SEC) SAS was employed. The SEC parameters were as follows: A 100.00 μl sample at 5.3 mg/ml was injected at a 0.10 ml/min flow rate onto a GE Superdex 200 Increase 10/300 column at 25°C. 852 successive 10 second frames were collected through the entire SEC elution. The data were normalized to the intensity of the transmitted beam and radially averaged; the scattering of the solvent-blank was subtracted.

The protein was recombinantly expressed in Escherichia coli.

p123 expressed protein (Gli123)
Mol. type		Protein
Organism		Mycoplasma mobile (strain ATCC 43663 / 163K / NCTC 11711)
Olig. state		Dimer
Mon. MW		123.9 kDa

UniProt		F8WJV6 (19-1128)
Sequence		FASTA