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Screening of diabetes-associated autoantigens and serum antibody profiles by phage display system
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Aims/Introduction: Phage display method is a crucial tool to
find novel clinically valuable diabetes-associated autoantigens, and
identify known autoantigen epitopes that are associated with diabetes;
could providing scientific support and guidance for the artificial
construction and synthesis of type I diabetes mellitus (T1DM) novel
biomarkers. Materials and Methods: The phage display system was
used for “bio-panning” of T1DM serum. Following by the sequencing of
the phage DNAs, the homologous sequences of the above fusion
heptapeptide were further investigated by BLAST to track the origin of
the polypeptide sequences. The antibody spectrum revealed new
T1DM-associated epitopes and antibodies. Results: A total of
1200 phage DNA were sequenced and 9 conserved polypeptide sequences were
collected. It was confirmed that the zinc transporter and islet amyloid
protease were among them.The conserved polypeptide sequence 8 and
another three distinctive polypeptide sequences derived from
Proteus were discovered. Furthermore, we expressed recombinant
proteins with homologous polypeptide sequences for the human islet
amyloid polypeptide (IAPP) polypeptide precursor human zinc transporter
8 (ZNT8). Through clinical sample detection for the serum from T1DM
(n=100) and T2DM (n=200) patients, results demonstrate the importance
and relevance of these polypeptides in the recognition and
classification of various forms of diabetes. Conclusion:Human
pancreatic and concurrent bacterial-derived protein antigens and their
epitopes were identified in this research by phage display system, which
is crucial for distinguishing different types of diabetes.
Title: Screening of diabetes-associated autoantigens and serum antibody profiles by phage display system
Description:
Aims/Introduction: Phage display method is a crucial tool to
find novel clinically valuable diabetes-associated autoantigens, and
identify known autoantigen epitopes that are associated with diabetes;
could providing scientific support and guidance for the artificial
construction and synthesis of type I diabetes mellitus (T1DM) novel
biomarkers.
Materials and Methods: The phage display system was
used for “bio-panning” of T1DM serum.
Following by the sequencing of
the phage DNAs, the homologous sequences of the above fusion
heptapeptide were further investigated by BLAST to track the origin of
the polypeptide sequences.
The antibody spectrum revealed new
T1DM-associated epitopes and antibodies.
Results: A total of
1200 phage DNA were sequenced and 9 conserved polypeptide sequences were
collected.
It was confirmed that the zinc transporter and islet amyloid
protease were among them.
The conserved polypeptide sequence 8 and
another three distinctive polypeptide sequences derived from
Proteus were discovered.
Furthermore, we expressed recombinant
proteins with homologous polypeptide sequences for the human islet
amyloid polypeptide (IAPP) polypeptide precursor human zinc transporter
8 (ZNT8).
Through clinical sample detection for the serum from T1DM
(n=100) and T2DM (n=200) patients, results demonstrate the importance
and relevance of these polypeptides in the recognition and
classification of various forms of diabetes.
Conclusion:Human
pancreatic and concurrent bacterial-derived protein antigens and their
epitopes were identified in this research by phage display system, which
is crucial for distinguishing different types of diabetes.
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Screening of diabetes-associated autoantigens and serum antibody profiles by phage display system
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