Current Proteomics, Vol. 1, No. 3, 2004
Contents
Recent Developments in Structural Proteomics: From
Protein Identifications and Structure Determinations to Protein-Protein Interactions
Pp.183-197
ELISA-based Protein Arrays: Multiplexed Sandwich
Immunoassays Pp.199-210
Ruo-Pan Huang, Ying Lin, Li-Pai Chen, Weimin Yang and
Ruochun Huang
Proteomics of Biofilm Bacteria Pp.211-219
Thierry Jouenne, Sebastien Vilain, Pascal Cosette and
Guy-Alain Junter
Proteomic Approaches Contributing to the Understanding of
Neurodegenerative Diseases: Focus on Alzheimer’s Disease Pp.221-229
Ephrem Engidawork and Gert Lubec
Fertilizome Project: Proteomics of Fertilization
Signaling - The Biological Bridge Between Gametogenesis and Embryogenesis Pp.231-246
Ken-ichi Sato, Claudio Sette, Manabu Kurokawa, Maria
Paola Paronetto, Tetsushi Iwasaki, Rafael A. Fissore and Yasuo Fukami
Thylakoid Membrane Proteome: Separation by HPLC and
Identification by Accurate Molecular Mass Determinations Pp.247-260
Lello Zolla, Anna Maria Timperio and Christian G. Huber
Abstracts
[Back to top]
Recent Developments in Structural Proteomics: From Protein Identifications and
Structure Determinations to Protein-Protein Interactions
Hsueh-Fen Juan, Hsuan-Liang Liu and Jyh-Ping Hsu
[Back to top] ELISA-based
Protein Arrays: Multiplexed Sandwich Immunoassays
Ruo-Pan Huang, Ying Lin, Li-Pai Chen, Weimin Yang and
Ruochun Huang
Protein arrays with ability to simultaneously detect multiple protein expression levels, protein-protein interactions, protein-DNA or RNA interactions, protein-small molecule interactions and protein modifications will be an excellent tool in biomedical discovery. A variety of technologies have been developed to meet this need. In general, these assay systems can be divided into two major categories: label-based approaches, and sandwich or enzyme linked immunosorbent assay (ELISA)-based approaches. The purpose of this review is to provide an overview of the principles and techniques of ELISA-based protein arrays, with particular emphasis on the use of ELISA-based protein arrays for detection of multiple protein expression levels.
[Back
to top] Proteomics of Biofilm Bacteria
Thierry Jouenne, Sebastien Vilain, Pascal Cosette and
Guy-Alain Junter
The formation of biofilms is a universal bacterial survival strategy. Biofilms occur on inert and living supports in natural environments and in industrial installations. Given their importance in various industrially relevant areas and in human health, numerous investigations have focussed on the particular physiology of these fixed microorganisms. It is now well recognised that bacteria present in biofilms behave quite differently from their planktonic counterparts. In particular, biofilm organisms are far more resistant to antimicrobial agents than are planktonic organisms. The mechanisms involved in the resistance of biofilm bacteria to antimicrobials are complex and still not fully understood. One of the hypotheses that suggested to explain the increased resistance of biofilms to antimicrobial agents assumes the existence of significant differences in gene expression. Although the expression of a limited number of genes appears to be altered during biofilm growth, a number of proteomics studies have revealed large physiological differences between free-living and biofilm bacteria. Moreover, multiple phenotypes were identified during the different stages of biofilm development. This review presents recent data on protein expression in sessile microorganisms that support the existence of a specific metabolic behaviour of biofilm bacteria.
[Back to top]
Proteomic Approaches Contributing to the Understanding of Neurodegenerative
Diseases: Focus on Alzheimer’s Disease
Ephrem Engidawork and Gert Lubec
With the advent of proteomic methods, a sudden switch from genomics to proteomics has been observed and indeed, in many cases no definite conclusions can be drawn from the nucleic acid data. Moreover, there is a long and unpredictable way from RNA to protein and differences between neurodegenerative disorders at the mRNA level could not be verified at the protein level. However, proteins carry out the ultimate function and thus the role of proteins is pivotal. Two-dimensional gel electrophoresis with in-gel digestion followed by mass spectrometric methods and subsequent quantification of proteins with specific software allow study of protein expression in a high-throughput way, identifying large series of proteins concomitantly. Furthermore, evaluation of protein expression by proteomic technologies does no longer rely upon the availability and specificity of antibodies. Significant proteomic approaches have been used to study degenerative diseases, including Alzheimer's disease, and many protein classes from signalling, metabolic, cytoskeleton, chaperone, antioxidant, and proteasome have been shown to be tentatively involved in pathological mechanisms. The aim of this review is to show what has been studied so far in the area using proteomic approaches, describing methodologies used including their potentials and limitations, and finally what still remains to be done. We are addressing only those methods and results necessary for discussing proteomic observations. The message of this review is that proteomics carries the potential to find important clues for pathogenesis of neurodegenerative diseases and to identify pharmacological targets, once the crucial problems such as analysis of hydrophobic and membrane proteins are solved.
[Back to top] Fertilizome
Project: Proteomics of Fertilization Signaling - The Biological Bridge Between
Gametogenesis and Embryogenesis
Ken-ichi Sato, Claudio Sette, Manabu Kurokawa, Maria Paola Paronetto, Tetsushi Iwasaki, Rafael A. Fissore and Yasuo Fukami
Fertilization is the biological bridge between gametogenesis and embryogenesis, by which sperm and eggs grow and mature, mate, and fuse with each other to give rise to the birth of a new individual(s). In this review, we address the current status of the knowledge in the field of fertilization, with a special focus on the role of maternal and paternal protein molecules such as tyrosine kinases, phospholipase C, and inositol trisphosphate receptor/Ca2+ channels in the establishment of intracellular Ca 2+ release, block to polyspermy, transition from meiotic to mitotic cell cycle, and nuclear fusion that are collectively called “sperm-induced egg activation”. We then discuss some proteomics approaches to analyze signaling events associated with sperm-induced egg activation. Protein profiling of subcellular microdomains and its differential display before and after fertilization, screening of fertilization-specific antigens by using a subtractive immunization scheme, and in vitro reconstitution of egg activation events using cell-free systems are now under investigation in our research team. These new experimental approaches, collectively termed “fertilizome project”, will be useful to understand the complexity of fertilization signaling, and will also be necessary for understanding and improving assisted reproduction and reproductive cloning techniques.
[Back to top] Thylakoid
Membrane Proteome: Separation by HPLC and Identification by Accurate Molecular
Mass Determinations
Lello Zolla, Anna Maria Timperio and Christian G. Huber
This review covers the vast array of methods that appeared in the last few years for separation and identification of thylakoid membrane proteins present in chloroplast, a good model for setting up analytical methods suitable for membrane proteins. Although the major method for protein separation is gel electrophoresis (GE), we will summarise in this review the results of several studies performed to develop a rapid and straightforward method based on high-performance liquid chromatography (HPLC) to resolve most of the antenna proteins of the two photosystems, photosystem I (PSI) and II (PSII) and identify them by intact molecular mass determination using electrospray ionization mass spectrometry (ESI-MS). The complex mixtures of these strongly hydrophobic membrane proteins are prefractionated by sucrose gradient ultracentrifugation in the first dimension followed by reversed-phase HPLC in the second dimension. The separation achieved is by far superior to that possible with GE. It is based on small differences in hydrophobicity of these very similar proteins. The correspondence between the intact molecular masses measured with those deduced from the DNA sequence enabled the identification of the different protein components of antenna complex. Isomeric forms of the proteins were readily revealed. On the contrary, peptide mass fingerprinting, commonly used for soluble proteins, does not seem to be very helpful for identification of these highly hydrophobic membrane proteins due to the limited number of peptides which can be obtained by proteolysis. Thus, separations and identifications of antenna proteins presented in this study may serve as reference for confident identification in future studies dealing with any membrane proteins.