Warning: Undefined array key "mm" in /www/wwwroot/www.ai-bt.com/si.php on line 10 Deprecated: trim(): Passing null to parameter #1 ($string) of type string is deprecated in /www/wwwroot/www.ai-bt.com/si.php on line 10 A differential scanning calorimetric study of the thermal unfolding of apo- and holo-cytochrome b562.

Literature DB >> 9568902

A differential scanning calorimetric study of the thermal unfolding of apo- and holo-cytochrome b562.

C R Robinson¹, Y Liu, R O'Brien, S G Sligar, J M Sturtevant.

Abstract

Cytochrome b562 is a four-helix-bundle protein containing a non-covalently bound b-type heme prosthetic group. In the absence of heme, cytochrome b562 remains highly structured under native conditions. Here we report thermodynamic data for the thermal denaturation of the holo- and apoproteins as determined by differential scanning calorimetry. Thermal denaturation of holocytochrome b562 is a highly reversible process, and unexpectedly does not involve dissociation of the heme prosthetic group. Thermal denaturation of the corresponding apoprotein, with the heme group chemically removed, remains a cooperative, reversible process. Apocytochrome b562 is substantially destabilized relative to the holoprotein: the t1/2 is more than ten degrees lower, and enthalpy and heat capacity changes are about one-half of the holoprotein values. However, the energetic parameters of apocytochrome b562 denaturation are within the range of observed values for small proteins.

Entities: Chemical Gene

Mesh：

Substances：

Year: 1998 PMID： 9568902 PMCID： PMC2143982 DOI： 10.1002/pro.5560070413

Source DB: PubMed Journal: Protein Sci ISSN： 0961-8368 Impact factor: 6.725

30 in total

1. Absence of the thermal transition in apo-alpha-lactalbumin in the molten globule state. A study by differential scanning microcalorimetry.

Authors: K Yutani; K Ogasahara; K Kuwajima
Journal: J Mol Biol Date: 1992-11-20 Impact factor: 5.469

2. Studies on cytochrome b-562 of Escherichia coli. I. Purification and crystallization of cytochrome b-562.

Authors: E Itagaki; L P Hager
Journal: J Biol Chem Date: 1966-08-25 Impact factor: 5.157

3. Protein folding. Matching speed and stability.

Authors: R L Baldwin
Journal: Nature Date: 1994-05-19 Impact factor: 49.962

4. Further examination of the intermediate state in the denaturation of the tryptophan synthase alpha subunit. Evidence that the equilibrium denaturation intermediate is a molten globule.

Authors: K Ogasahara; E Matsushita; K Yutani
Journal: J Mol Biol Date: 1993-12-20 Impact factor: 5.469

5. Partially folded states of equine lysozyme. Structural characterization and significance for protein folding.

Authors: H Van Dael; P Haezebrouck; L Morozova; C Arico-Muendel; C M Dobson
Journal: Biochemistry Date: 1993-11-09 Impact factor: 3.162

6. Electrostatic stabilization in four-helix bundle proteins.

Authors: C R Robinson; S G Sligar
Journal: Protein Sci Date: 1993-05 Impact factor: 6.725

7. Design and synthesis of multi-haem proteins.

Authors: D E Robertson; R S Farid; C C Moser; J L Urbauer; S E Mulholland; R Pidikiti; J D Lear; A J Wand; W F DeGrado; P L Dutton
Journal: Nature Date: 1994-03-31 Impact factor: 49.962

8. Energetics of heme binding to native and denatured states of cytochrome b562.

Authors: C R Robinson; Y Liu; J A Thomson; J M Sturtevant; S G Sligar
Journal: Biochemistry Date: 1997-12-23 Impact factor: 3.162

9. Similarities in structure between holocytochrome b5 and apocytochrome b5: NMR studies of the histidine residues.

Authors: C D Moore; O N al-Misky; J T Lecomte
Journal: Biochemistry Date: 1991-08-27 Impact factor: 3.162

10. Comparison of the conformational stability of the molten globule and native states of horse cytochrome c. Effects of acetylation, heat, urea and guanidine-hydrochloride.

Authors: Y Hagihara; Y Tan; Y Goto
Journal: J Mol Biol Date: 1994-04-01 Impact factor: 5.469

6 in total

A differential scanning calorimetric study of the thermal unfolding of apo- and holo-cytochrome b562.

1. Absence of the thermal transition in apo-alpha-lactalbumin in the molten globule state. A study by differential scanning microcalorimetry.

2. Studies on cytochrome b-562 of Escherichia coli. I. Purification and crystallization of cytochrome b-562.

3. Protein folding. Matching speed and stability.

4. Further examination of the intermediate state in the denaturation of the tryptophan synthase alpha subunit. Evidence that the equilibrium denaturation intermediate is a molten globule.

5. Partially folded states of equine lysozyme. Structural characterization and significance for protein folding.

6. Electrostatic stabilization in four-helix bundle proteins.

7. Design and synthesis of multi-haem proteins.

8. Energetics of heme binding to native and denatured states of cytochrome b562.

9. Similarities in structure between holocytochrome b5 and apocytochrome b5: NMR studies of the histidine residues.

10. Comparison of the conformational stability of the molten globule and native states of horse cytochrome c. Effects of acetylation, heat, urea and guanidine-hydrochloride.

1. Stably folded de novo proteins from a designed combinatorial library.

2. Cold instability of aponeocarzinostatin and its stabilization by labile chromophore.

3. Replacement of the Distal Histidine Reveals a Noncanonical Heme Binding Site in a 2-on-2 Hemoglobin.

4. Conformational properties of native sperm whale apomyoglobin in solution.

5. Dynamics of Dystrophin's Actin-Binding Domain.

6. Domain-swapped cytochrome cb₅₆₂ dimer and its nanocage encapsulating a Zn-SO₄ cluster in the internal cavity.