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. 2018 Dec 17;2018:9538193. doi: 10.1155/2018/9538193

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Copyright © 2018 María de J. López-López et al.

This is an open access article distributed under the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

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Secondary and tertiary structure of enolases. (a) Far-UV circular dichroism spectra; black cross: Streptococcal surface enolase; red line: P. falciparum enolase (dimer); red dashed line: P. falciparum enolase (monomer);pink line with asterisks: S. pyogenes enolase (TME buffer); pink asterisks: S. pyogenes enolase (Glycine buffer); green circles: S. cerevisiae enolase; blue closed squares: apo-HpEno (Tris-HCl); blue open squares: holo-HpEno (Tris-HCl); blue closed triangles: apo-HpEno (potassium phosphate); blue open triangles: holo-HpEno (potassium phosphate). (b) Fluorescence emission spectra for the excitation wavelength of 280 nm; Green closed circles: S. cerevisiae enolase (Tris-acetate); green open circles: S. cerevisiae enolase (Tris-HCl); blue closed squares: apo-HpEno(Tris-HCl); blue stars: apo-HpEno (Tris-acetate). (c) Fluorescence emission spectra for the excitation wavelength of 295 nm; red line: P. falciparum enolase; green open circle: S. cerevisiae enolase (Tris-HCl); blue closed squares: apo-HpEno(Tris-HCl); blue stars: apo-HpEno (Tris-acetate).