Current Proteomics
ISSN: 1570-1646
Current Proteomics
Volume 4 Number 2, July 2007
Contents
Proteomic Study of Micro-Algae: Sample Preparation
for Two Dimensional Gel Electrophoresis and De Novo
Peptide Sequencing Using MALDI-TOF MS Pp. 67-78
F.W-F. Lee and S.C-L. Lo
[Abstract]
Proteomic Advances in Phytopathogenic Fungi
Pp. 79-88
F.J. Fernández-Acero, M. Carbú, C. Garrido,
I. Vallejo and J.M. Cantoral
[Abstract]
Cerebrospinal Fluid Proteomes: From Neural Development
to Neurodegenerative Diseases Pp. 89-106
C. Parada, M. Parvas and D. Bueno
[Abstract]
Antigenicity Prediction in Melittin: Possibilities
of in Drug Development from Apis dorsata
Pp. 107-114
V.S. Gomase and S.S. Changbhale
[Abstract]
Safe and Convenient Fluorescent Stain Imager for Proteome
Analysis Pp. 115-120
T. Terakawa, N. Keicho, C. Uchida and T. Uchida
[Abstract]
Abstracts
[Back to top]
Proteomic Study of Micro-Algae: Sample Preparation for Two
Dimensional Gel Electrophoresis and De Novo Peptide
Sequencing Using MALDI-TOF MS
F.W-F. Lee and S.C-L. Lo
Proteins are the major players in most processes of living
cells and study of the proteome has great relevance to investigations
on cells and organisms at the molecular level. 2-DE is a core
and powerful proteomic technique to study protein expression
and function in living organisms and it allows a fast overview
of changes that occurred in cells at the proteome level. Although
data on DNA sequences from large scale genomic sequencing
projects has greatly facilitated the identification and characterization
of proteins, genomic sequences of many organisms, including
that of many microalgae are still unknown. Thus, de novo
protein/peptide sequencing techniques are important for acquiring
amino acid sequences of proteins from organisms with incomplete
genome data. Take dinoflagellates as an example of micro-algae
for discussion purposes, they are the major causative agents
of harmful algal blooms (HABs). Lack of well described genome
information of dinoflagellates has limited progress of proteomic
studies on these organisms. Nevertheless, 2-DE combined with
de novo protein/peptide sequencing could provide
an alternative route for identification and annotating proteins
of interest in these organisms. However, preparation of high-quality
samples of dinoflagellate cell extracts for 2-DE analysis
is difficult due to the presence of high endogenous levels
of nucleic acids, polysaccharides, salts, pigments, and other
interfering compounds. Thus, an optimized protocol of sample
preparation is a pre-requisite for obtaining satisfactory
and reproducible 2-DE profiles. In light of these perceived
problems, we had reviewed current methods available for preparing
dinoflagellate samples for 2-DE analysis with some working
alternatives from the authors’ laboratory. Moreover,
de-novo protein/peptide sequencing methods by MALDI-TOF
MS assisted by effective derivatization protocols were also
described.
[Back to top]
Proteomic Advances in Phytopathogenic Fungi
F.J. Fernández-Acero, M. Carbú, C. Garrido,
I. Vallejo and J.M. Cantoral
Phytopathogenic fungi are organisms responsible for several
plant diseases in different crops around the world, causing
very important economic losses to the farmers. Fungi have
a complicated life cycle, normally with asexual and sexual
reproduction that involves the formation of different reproductive
structures. Moreover, during plant disease, fungi produce
different components that are essential to complete the infection
process (enzymes, toxins, etc) and are named “pathogenicity
factors”.
Two dimensional gel electrophoresis (2-DE) has been widely
used to study the proteome of a good number of microorganisms.
However, few of them have been carried out to study the proteome
of phytopathogenic fungi, mainly due to the difficulty of
obtaining fungal protein extracts and/or the lack of available
fungal protein databases. This review shows the strategies
that can be addressed to overcome those problems and how different
approaches have resulted to be useful in (i) obtaining the
proteomic maps of several phytopathogenic fungi, (ii) determining
fungal proteins involved in the formation of infective structures
and (iii) studying the production of extracellular proteins
or pathogenicity factors in phytopathogenic fungi. Fungal
proteomic is still at an early stage, but recent reports show
that it is a potential tool for identifying pathogenicity
factors, therapeutic targets and for basic research.
[Back to top]
Cerebrospinal Fluid Proteomes: From Neural Development
to Neurodegenerative Diseases
C. Parada, M. Parvas and D. Bueno
Global characterisation of proteins and the comparison between
proteomes is providing new insights into general biological
structures and processes, as well as between physiological
and pathological conditions. During both embryonic development
and adult life, brain cavities and ventricles are filled with
a complex protein-rich fluid, the cerebrospinal fluid (CSF).
In the last few years, it has been suggested that adult CSF
has a key function as a fluid pathway for delivering diffusible
signals to the brain, thus affecting the behaviour of specific
brain parenchyma cells, particularly the putative neural stem
cells. Accordingly, some pathologies that affect the central
nervous system (CNS), such as neurodegenerative diseases and/or
neurological disorders, are reflected in CSF protein content,
either as a cause or as a consequence. Adult CSF is considered
to be the successor of embryonic CSF (E-CSF). Most of the
proteins contained within E-CSF, as analysed in avians (chick)
and mammals (rat and human), are also detected in adult humans,
suggesting that some of their roles in CNS cell behaviour
are similar. Despite the heterogeneity of the currently available
data, which is due to technical differences in the proteomic
analyses, the use of different model systems and the great
variety of sample sources, it is increasingly clear that this
fluid regulates the behaviour of neural stem cells throughout
development and during adult life, thus suggesting a possible
approach to brain cell therapies. This review focuses on current
data regarding CSF proteomes in relation to CSF functions
in both physiological and pathological conditions, as well
as on CSF manufacture.
[Back to top]
Antigenicity Prediction in Melittin: Possibilities
of in Drug Development from Apis dorsata
V.S. Gomase and S.S. Changbhale
The bee venom is used for treating a wide variety of conditions
from acute tendonitis to chronic back pain to rheumatoid arthritis
(RA). The major treatment is gene therapy or recombinant DNA
vaccines involved in targeting multiple antigenic components
to direct and empower the immune system to protect the host
from infection. Limitations of therapy for the treatment of
patients suffering from various adverse reaction and contraindications
are always experienced. Antigenic epitopes on melittin protein
of Apis dorsata are important determinants of protection
against rheumatoid arthritis. As our knowledge of the immune
responses to a protein antigen progressed, it became clear
that the whole protein is not necessary for raising the immune
response, but small segments as 4-AILKVLSTGLPALIS-18 of protein
called the antigenic determinants or the epitopes, are sufficient
for eliciting the desired immune response. Immunization cassettes
should be capable of immunizing broad immunity against both
humoral and cellular epitopes, thus giving vaccines the maximum
ability to deal with A. dorsata immune escape against
rheumatoid arthritis.
[Back to top]
Safe and Convenient Fluorescent Stain Imager for Proteome
Analysis
T. Terakawa, N. Keicho, C. Uchida and T. Uchida
We have produced a safe and convenient “fluorescence
imager” to observe the protein bands and spots in the
polyacrylamide gel stained by the fluorescent stain. Coomassie
brilliant blue (CBB) and the argentation or silver stain method
have been used usually for this staining. The staining of
the gel using a fluorescent stain, such as SYPRO Ruby was
developed recently. This fluorescent stain has more advantages
compared to the CBB and silver stain method. The most common
fluorescent stain used for observation of the protein bands
analyzed by polyacrylamide gel electrophoresis is SYPRO Ruby.
To detect the SYPRO Ruby stained bands, an ultraviolet (UV)
transilluminator or a large and expensive laser scanner is
required. A UV transilluminator is usually used because fluorescent
stain scanners are cumbersome and expensive for this purpose.
Although UV light is harmful to eyes and skin, it has been
used usually to identify and excise the target protein bands
and spots in the gel. In addition to the need for, protection
of the users, UV light damages the proteins.
We have produced a convenient and safer fluorescent stained
gel imager to avoid the above problems. The sensitivity of
our device is as high as that of the laser scanner, the excitation
light is not harmful to the human body and does not damage
proteins. Additionally it is possible to produce various sizes
of devices required for this purpose.
|
