PMID- 26963430
OWN - NLM
STAT- MEDLINE
DCOM- 20170303
LR  - 20170303
IS  - 1873-2682 (Electronic)
IS  - 1011-1344 (Linking)
VI  - 158
DP  - 2016 May
TI  - Fluorescence investigations on choline phospholipid binding and chemical 
      unfolding of HSP-1/2, a major protein of horse seminal plasma.
PG  - 89-98
LID - S1011-1344(15)30108-1 [pii]
LID - 10.1016/j.jphotobiol.2016.02.025 [doi]
AB  - Seminal fibronectin type-II (Fn-II) proteins interact with choline phospholipids 
      present on the sperm plasma membrane and play a crucial role in sperm 
      capacitation. Crystal structure of phosphorylcholine (PrC) complex of PDC-109, 
      the major bovine Fn-II protein, together with fluorescence spectroscopic studies 
      has shown that tryptophan residues are crucial for its specific interaction with 
      choline phospholipids. In the present study, the heterogeneity and 
      microenvironment of tryptophan residues in HSP-1/2, a major protein of horse 
      seminal plasma (which is homologous to PDC-109) were investigated in the native 
      state, in the presence of PrC and phosphatidylcholines (PCs) with short (valeryl, 
      C-5) and long (myristoyl, C-14) chains, and upon denaturation using fluorescence 
      quenching, time-resolved fluorescence and red-edge excitation shift (REES) 
      measurements. The results obtained show that the environment of tryptophan 
      residues in HSP-1/2 is more heterogeneous as compared to that in PDC-109. Binding 
      of choline containing ligands afforded a protection to the tryptophan residues 
      with the shielding order being: PrC</=divalaroyl PC<dimyristoyl PC. REES value 
      obtained for HSP-1/2 (3.5nm) is smaller than that of observed for PDC-109 (4nm) 
      and binding to PrC and DVPC reduced the REES to 1nm. HSP-1/2 exhibits only 
      partial unfolding with chemical denaturants with no cooperativity, whereas 
      complete unfolding was observed in the presence of 10mM dithiothreitol, 
      indicating that disulfide linkages prevent complete unfolding of the protein. In 
      the presence of PrC the transition midpoints shifted to higher concentrations of 
      the denaturant together with a broadening of the sigmoidal transitions, 
      indicating that ligand binding as well as polydispersity modulate the unfolding 
      process.
CI  - Copyright (c) 2016 Elsevier B.V. All rights reserved.
FAU - Kumar, C Sudheer
AU  - Kumar CS
AD  - School of Chemistry, University of Hyderabad, Hyderabad 500046, India.
FAU - Sivaramakrishna, D
AU  - Sivaramakrishna D
AD  - School of Chemistry, University of Hyderabad, Hyderabad 500046, India.
FAU - Ravi, Sanjay K
AU  - Ravi SK
AD  - Animal Reproduction Laboratory, ICAR-National Research Centre on Equines, Bikaner 
      334001, India.
FAU - Swamy, Musti J
AU  - Swamy MJ
AD  - School of Chemistry, University of Hyderabad, Hyderabad 500046, India. Electronic 
      address: mjswamy@uohyd.ac.in.
LA  - eng
PT  - Journal Article
DEP - 20160303
PL  - Switzerland
TA  - J Photochem Photobiol B
JT  - Journal of photochemistry and photobiology. B, Biology
JID - 8804966
RN  - 0 (Heat-Shock Proteins)
RN  - 0 (Phospholipids)
RN  - N91BDP6H0X (Choline)
SB  - IM
MH  - Animals
MH  - Choline/*metabolism
MH  - Heat-Shock Proteins/chemistry/*metabolism
MH  - Horses
MH  - Male
MH  - Phospholipids/*metabolism
MH  - Protein Binding
MH  - Protein Unfolding
MH  - Semen/*chemistry
MH  - Spectrometry, Fluorescence/*methods
OTO - NOTNLM
OT  - Capacitation
OT  - Chaperone
OT  - Chemical unfolding
OT  - Fluorescence quenching
OT  - Polydispersity
OT  - Red edge excitation shift
EDAT- 2016/03/11 06:00
MHDA- 2017/03/04 06:00
CRDT- 2016/03/11 06:00
PHST- 2015/10/22 00:00 [received]
PHST- 2016/02/08 00:00 [revised]
PHST- 2016/02/11 00:00 [accepted]
PHST- 2016/03/11 06:00 [entrez]
PHST- 2016/03/11 06:00 [pubmed]
PHST- 2017/03/04 06:00 [medline]
AID - S1011-1344(15)30108-1 [pii]
AID - 10.1016/j.jphotobiol.2016.02.025 [doi]
PST - ppublish
SO  - J Photochem Photobiol B. 2016 May;158:89-98. doi: 
      10.1016/j.jphotobiol.2016.02.025. Epub 2016 Mar 3.