 Press Release
Angewandte Chemie International Edition 2009, 48,
doi: 10.1002/anie.200804734 Nr. 04/2009 Enzyme with a Sugar AntennaResearchers achieve semisynthesis of homogeneous glycoproteinsContact: Carlo Unverzagt, Universität Bayreuth (Germany)
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Semisynthesis of a Homogeneous Glycoprotein Enzyme: Ribonuclease C More
than half of all human proteins, as well as many important
pharmaceutical agents, are glycoproteins, which means that they contain
sugar components. In general, natural glycoproteins do not have a
homogeneous sugar component. With modern purification techniques, it is
practically impossible to isolate sufficient quantities of homogeneous
glycoproteins for systematic biomedical studies. Synthesis in the lab is
a good alternative—but also a very complex task. As they report in the
journal Angewandte Chemie, scientists led by Carlo Unverzagt at
the University of Bayreuth (Germany) have now successfully used a new
strategy to synthesize ribonuclease C (RNase C), a glycosylated bovine
pancreatic enzyme.
© Wiley-VCH
Sugar
components play an important role in the water solubility, stability, and
folding of glycoproteins. In addition, they participate in molecular
-recognition processes, such as cell adhesion or the interaction of host
cells with pathogens. The same protein with different sugar moieties can
thus have different functions. RNase is an enzyme that occurs in various
glycosylated forms. Because this enzyme has been intensively
investigated before, it makes an interesting model system for research.
RNase C contains a complex sugar component in the form of a double-ended
“antenna”.
The conventional
solid-phase synthesis used to build up peptides one amino acid at a time
is much too complex for long peptide chains and sometimes doesn’t work
at all because of side reactions. Unverzagt and his team thus built up
RNase C sequentially from several fragments, connecting them by using
“native chemical ligation”. In this technique, one peptide fragment is
attached to the terminal cysteine group (sulfur-containing amino acid)
of a second peptide fragment by means of a thioester group—a
selective reaction that results in a natural peptide bond.
The
researchers used solid-phase synthesis to make the critical peptide
fragment that has the sugar antenna. Another fragment was obtained
bacterially by means of a method derived from protein splicing. In this
process, a protein sequence (intein) is autocatalytically split off from
a fusion protein generated in a cell culture. The difficulty: as well as
a terminal cysteine group, this protein fragment contains seven
additional cysteines. Their sulfur–hydrogen groups are extremely
reactive and sensitive toward oxidation. In order to protect them, they
were “sealed off” as mixed disulfides. These protective groups could be
easily removed afterwards.
Thanks
to sophisticated techniques, the team was finally able to correctly
attach the individual fragments, fold the enzyme into its natural form,
and correctly couple the cysteines into disulfide bridges to form a
functional RNase C.
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