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Macrocypins,afamilyofcysteineproteaseinhibitors from
the basidiomyceteMacrolepiota procera
Jerica Sabotic
ˇ
1
, Tatjana Popovic
ˇ
1
, Vida Puizdar
2
and Joz
ˇ
e Brzin
1
1 Department of Biotechnology, Joz
ˇ
ef Stefan Institute, Jamova 39, Ljubljana, Slovenia
2 Department of Biochemistry and Molecular and Structural Biology, Joz
ˇ
ef Stefan Institute, Jamova 39, Ljubljana, Slovenia
Introduction
Papain-like cysteine proteases are widespread in organ-
isms ranging from bacteria to humans. They play impor-
tant roles in many facets of physiology, and
dysregulation of proteolytic activity can lead to a variety
of pathologies, including cancer, rheumatoid arthritis,
osteoarthritis and neurological disorders [1,2]. The most
important regulators ofprotease activity are specific
protease inhibitors. In addition to their considerable
potential in diverse medical applications, protease inhib-
itors have been studied as tools for analysing proteolytic
mechanisms and protein–protein interactions, and as
biocidal agents against various organisms. There are
several groups of inhibitors, mainly from animal and
plant origins, that specifically inhibit papain-like cyste-
ine proteases [3,4]. The first cysteineprotease inhibitor
isolated from higher fungi was clitocypin from the
basidiomycete Clitocybe nebularis [5]. Clitocypin is a
16.8-kDa protein lacking cysteine and methionine resi-
Keywords
basidiomycetes; clitocypin; cysteine
protease; mycocypin; protease inhibitor
Correspondence
J. Sabotic
ˇ
, Department of Biotechnology,
Joz
ˇ
ef Stefan Institute, Jamova 39, 1000
Ljubljana, Slovenia
Tel: +386 1 477 3754
Fax: +386 1 477 3594
E-mail: Jerica.Sabotic@ijs.si
Note
The nucleotide sequences reported in this
paper have been deposited in the
DDBI ⁄ EMBL ⁄ GenBank databases under
accession numbers FJ495239, FJ495240,
FJ495241, FJ495242, FJ495243, FJ495244,
FJ495245, FJ495246, FJ495247, FJ495248,
FJ495249, FJ495250, FJ548751 and
FJ548752
(Received 25 March 2009, revised 22 May
2009, accepted 9 June 2009)
doi:10.1111/j.1742-4658.2009.07138.x
A new familyofcysteineproteaseinhibitorsfromthebasidiomycete Mac-
rolepiota procera has been identified and thefamily members have been
termed macrocypins. These macrocypins are encoded by afamilyof genes
that is divided into five groups with more than 90% within-group sequence
identity and 75–86% between-group sequence identity. Several differences
in the promoter and noncoding sequences suggest regulation of macrocypin
expression at different levels. High yields of three different recombinant
macrocypins were produced by bacterial expression. The sequence diversity
was shown to affect the inhibitory activity ofmacrocypins,the heterolo-
gously expressed macrocypins belonging to different groups showing differ-
ences in their inhibitory profiles. Macrocypins are effective inhibitors of
papain and cysteine cathepsin endopeptidases, and also inhibit cathepsins
B and H, which exhibit both exopeptidase and endopeptidase activities.
The cysteineprotease legumain is inhibited by macrocypins with the excep-
tion of one representative that exhibits, instead, a weak inhibition of serine
protease trypsin. Macrocypins exhibit similar basic biochemical characteris-
tics, stability against high temperature and extremes of pH, and inhibitory
profiles similar to those of clitocypin from Clitocybe nebularis, the sole rep-
resentative ofthe I48 protease inhibitor family in the
MEROPS database.
This suggests that they belong to the same merops familyofcysteine prote-
ase inhibitors, the mycocypins, and substantiates the establishment of the
I48 protease inhibitor family.
Abbreviations
AMC, 7-amido-4-methylcoumarin; Clt, clitocypin; Mcp1, 2, 3, 4, 5, macrocypin 1, 2, 3, 4, 5; rMcp1, 3, 4, recombinant macrocypin 1, 3, 4; Z,
benzyloxycarbonyl.
4334 FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS
dues, which, on account of its unique characteristics,
was assigned to a new familyofcysteineprotease inhibi-
tors, I48 in the merops database inhibitor classification,
also named mycocypins. Its profile of inhibition differs
from those of other then known families ofcysteine pro-
tease inhibitors. Clitocypin inhibits papain, cathepsins L
and K, legumain and bromelain, but is inactive against
cathepsin H, trypsin and pepsin. Clitocypin is encoded
by a small familyof genes that show sequence hetero-
geneity, which does not affect its inhibitory activity.
In addition to a defensive role, a regulatory role in
mushroom endogenous proteolytic systems was pro-
posed, based on the specific inhibition of several puta-
tive fungal cysteine proteases [5–7].
The proteolytic potential of higher fungi is consid-
erable in terms ofthe number and diversity of prote-
ases they contain [8], and basidiomycetes are a rich
source of novel proteolytic enzymes and their inhibi-
tors [5,8]. As a result ofa study carried out to inves-
tigate the extent and function ofthe I48 inhibitor
family that to date includes only one characterized
member, we report a novel familyofcysteine prote-
ase inhibitorsfrom basidiocarps, or fruiting bodies,
of thebasidiomyceteMacrolepiota procera, and have
characterized some of its natural and recombinant
members.
Results
Isolation of cysteine-protease inhibitors from
M. procera
Cysteine proteaseinhibitors were purified from basid-
iocarps of M. procera by a method similar to that used
to purify clitocypin from basidiocarps of C. nebularis,
which included hydrophobic interaction, ion-exchange
and papain affinity chromatographies [5,9]. The inhibi-
tory proteins were separated on SDS–PAGE under
denaturing, nonreducing, conditions into two bands
corresponding to apparent molecular masses of 21 and
17 kDa (Fig. 1). The 43-residue N-terminal sequence
for the former protein (Fig. 2) was 42% identical and
58% similar to the N-terminal sequence of clitocypin.
The new 21-kDa cysteineprotease inhibitor has been
named macrocypin (
Macrolepiota proceracysteine pro-
tease
inhibitor, Mcp). The N-terminal sequence for the
lower-molecular-mass protein could not be determined,
possibly because ofa blocked N terminus. The pres-
ence ofa protein of similar size to that of clitocypin
and purified by the same procedure, and with similar
biochemical properties, indicated the presence ofa clit-
ocypin-like cysteineprotease inhibitor in M. procera
[5,6]. This was confirmed at the genetic level by geno-
mic DNA dot-blot analysis and by amplification of
partial clitocypin-like gene sequences. The partial
sequences ofthe clitocypin-like genes from M. procera
are more than 90% identical to those of clitocypin
at the nucleotide level (see Supplementary Data in
Doc. S1 and Doc. S2 and Fig. S1 and S2).
Cloning and analysis of macrocypin cDNA and
gene sequences
The N-terminal sequence (H
2
N-GLEDGLYTIRHLVE
GQPPNIPGGMYASSKDGKDXPVTAEPPLP) and
the sequence of an internal peptide fragment obtained
by digestion with cyanogen bromide (H
2
N-YIP-
RKVFK) were used to design degenerate primers
(Table S1). Degenerate primers and M. procera cDNA
synthesized from total RNA as template were used to
obtain a specific macrocypin sequence. This was then
used to design specific nested primers for use in
Genome walking and 3¢ RACE methods.
Two fragments were cloned fromthe two genomic
libraries obtained by the Universal Genome Walker kit
(Clontech, Heidelberg, Germany), using mcp gene-spe-
cific antisense primers – Pr4 (1000 bp) and Pr3
(204 bp). Each corresponds to the mcp 5¢ UTR and
promoter regions. Sequences spanning the 5¢ coding
region ofthe mcp gene were not identical (Fig. S3),
suggesting that more than one gene encoding macrocy-
pin is present in the M. procera genome, each of which
has its corresponding promoter. Both promoter
sequences have a typical TATA box (TATAAAA)
present at position )85, and a putative transcription
initiation site (CTAGTCC) at position )55, indicating
Fig. 1. SDS–PAGE analysis ofthe natural cysteineprotease inhibi-
tors clitocypin (nClt) and macrocypin (nMcp). Clitocypin (from Clito-
cybe nebularis) and macrocypin (from Macrolepiota procera)
purified from basidiocarps were analyzed under nonreducing, dena-
turing conditions and stained with Coomassie Blue. Lane M,
protein molecular mass markers.
J. Sabotic
ˇ
et al. Fungal cysteineprotease inhibitors
FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS 4335
transcriptional activity of macrocypin genes. The loca-
tion ofthe TATA box at a position 30 nucleotides
upstream fromthe putative transcription-initiation site
is in accordance with the locations found in several
other fungal genes, which are usually within 30–60
nucleotides ofthe transcription start site [10].
To obtain the coding and 3¢ UTR regions ofthe mcp
mRNA, we used the 3¢ RACE method with mcp-specific
sense primers that differentiate between the two
sequences obtained by genome walking. Partial
sequences corresponding to promoter Pr4 showed two
different lengths ofthe 3¢ UTR (66 nucleotides and 87
nucleotides). Sequences corresponding to promoter Pr3
showed even more variation in 3¢UTR length (64, 69, or
88 nucleotides), indicating the possibility of macrocypin
translation being regulated via the 3¢ UTR [11]. There is
no typical polyadenylation signal present in the 3¢ UTR.
The genomic sequence corresponding to the 3¢ UTR was
amplified fromthe two genomic libraries created using
the Universal Genome Walker kit (Clontech), using
mcp-specific sense primers. Two fragments, spanning
175 and 151 bp downstream ofthe stop codon, were
obtained that were identical to the overlapping sequence
of the 3¢UTR region amplified from M. procera cDNA,
corresponding to the promoter fragment Pr4.
The full-length gene and cDNA sequences of macro-
cypin were obtained, using primers annealing to the 5¢
UTR and 3¢ UTR regions and genomic DNA or first-
strand cDNA synthesized fromthe total RNA of
M. procera as templates. Several different gene and
cDNA sequences were amplified, all of which, how-
ever, shared the same gene structure. The mcp genes
were found to be composed of four exons and three
short introns with exon–intron boundaries matching
the consensus splice sites predicted for eukaryotic
genes [10]. Based on a sequence identity matrix of the
deduced amino acid sequences, we divided the
obtained sequences into five groups, naming them
macrocypin 1–5. Sequence identity at the deduced
amino acid sequence level between the five macrocypin
groups was 75–86%, while sequences within groups
exhibited more than 90% sequence identity.
The length ofthe macrocypin 1 (Mcp1) deduced
amino acid sequence was 169 residues, with a molecu-
lar mass of 19 193 Da, while the length ofthe repre-
sentatives ofthe other four groups was 167 residues,
with molecular masses between 18 770 and 19 031 Da.
Single cysteines were present in Mcp1, macrocypin 4
(Mcp4) and macrocypin 5 (Mcp5) (C106), none in
macrocypin 2 (Mcp2) and none or one (C75) in macro-
Fig. 2. Diversity in thecysteineprotease inhibitor macrocypin family. Amino acid sequences deduced from macrocypin (Mcp) genes (pref-
aced by g) and from cDNA sequences (prefaced by c) belonging to different groups (macrocypins 1–5) are aligned with the N-terminal
sequence determined for the natural macrocypin (nMcp) isolated from basidiocarps ofMacrolepiota procera. Identical residues in at least 9
of 11 sequences (80 %) are highlighted in dark gray and similar residues are highlighted in light gray. Sequences corresponding to clones
used for the heterologous expression of macrocypins are indicated in bold. Residues subjected to positive evolution, as determined using
the Datamonkey rapid detection of positive selection web server [20], are marked with an asterisk.
Fungal cysteineproteaseinhibitors J. Sabotic
ˇ
et al.
4336 FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS
cypin 3 (Mcp3). All the sequences showed high con-
tents of proline, of around 9.2% (the average overall
protein content is 4.7 %), of tryptophan, of 3.6%
(average 1.1 %) and of tyrosine, of 6.0–6.6% (average
2.9%), and low leucine contents of around 3.6% (aver-
age 9.7%) [12]. With the exception of Mcp3, macrocy-
pin sequences also showed a high glycine content of
around 9.8% (average 6.9%).
Variability in the sequences of macrocypin genes
The diversity observed for the macrocypin coding
sequences was greater than that for clitocypins [7]. The
coding sequence, composed of four exons, was 507 bp
for Mcp1 and 501 bp for the other macrocypins. The
deduced amino acid sequence for Mcp1 was thus two
amino acids longer, because of an insertion near the N
terminus. The lengths ofthe four exons were 147 or
153, 212, 70 and 75 bp, and ofthe three introns were
56, 49 or 51, and 50 or 54 bp. The sequence diversity
was equally distributed in introns and in exons
(Fig. S3). The second intron showed the greatest diver-
sity in sequence and was 2 bp shorter in Mcp3 and
Mcp5. The third intron was the most highly conserved
of the three, with the exception of Mcp3, where it was
4 bp shorter. Diversity in the coding sequence was dis-
tributed throughout the sequence (Fig. 2) and this was
caused by one, two or three nucleotide substitutions
that resulted in 47 variable codons at the level of the
deduced amino acid sequences. Some of these codons
subjected to positive selection (codons 18, 85, 89, 105,
107 and 116) were identified at the P < 0.05 level
(Fig. 2). Codons under negative selection (31 codons
identified) appeared to be evenly distributed along the
whole mcp genes without particular clustering. The few
positively selected sites in the mcp genes may provide
insights into the physiological role ofmacrocypins, as
these sites are more likely to be involved in interac-
tions with other proteins.
Similarity searches for the macrocypin sequences
against NCBI databases using blastn [13] revealed no
significant similarities (cut-off e < 0.1). tblastn
searches, by contrast, found significant sequence simi-
larity to the clitocypin cysteineprotease inhibitor
annotated in the Laccaria bicolor S238N-H82 genome
[14]. There was 39–44% sequence similarity and
26–29% sequence identity for different macrocypin
sequences, the highest being with that of Mcp5. No
significant similarities were found for the macrocypin
sequences in the completed and unfinished archaeal or
bacterial genomes or in other eukaryotic genomes,
which is probably the result of low overall sequence
similarity between mycocypins.
Alignment of macrocypin deduced amino acid
sequences with clitocypin sequences showed 17–21%
sequence identity (Fig. 3). The N-terminal halves of
the sequences showed more similarity. The higher
molecular masses relative to the clitocypins are caused
by a few insertions and deletions of two to seven
amino acids, distributed along the sequence. Another
important difference between the macrocypin and clit-
ocypin sequences was the presence ofacysteine residue
Fig. 3. Alignment of mycocypin deduced amino acid sequences. Deduced amino acid sequences of macrocypins belonging to each of the
five groups are aligned with three representative clitocypin deduced amino acid sequences (GenBank accession numbers: gClt-Kras,
AAZ78483.1; cClt-Kras, AAZ78481.1; and cClt-Vrh, AAZ78482.1). Sequences are prefaced by g or c to indicate whether they are deduced
from genomic or cDNA sequences. Identical residues in at least seven ofthe eight sequences (90 %) are highlighted in dark grey and similar
residues are highlighted in light grey.
J. Sabotic
ˇ
et al. Fungal cysteineprotease inhibitors
FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS 4337
in most macrocypins, and of several histidine and
methionine residues in all the macrocypin sequences,
all of which are absent in clitocypin. High proline and
glycine contents were, by contrast, common to both
macrocypins and clitocypin.
Heterologous expression of macrocypins
The cDNA clones that were available for Mcp1, Mcp3
and Mcp4 (marked in bold in Fig. 2), were cloned into
expression vectors ofthe pET System (Novagen, Madi-
son, WI, USA) for heterologous expression in Escheri-
chia coli (Fig. S4). Macrocypin 1a (Mcp1a) and
macrocypin 3a (Mcp3a) cDNA clones were each
cloned into two expression vectors (pET3a and
pET11a) to assess their expression in the bacterial
expression system. Heterologous expression of recom-
binant Mcp1 (rMcp1) was higher with the pET11a
expression vector construct, while that of recombinant
Mcp3 (rMcp3) was higher using pET3a. The amounts
of both recombinant proteins were highest 6 h after
induction (data not shown). The macrocypin 4a
(Mcp4a) cDNA clone was introduced into the pET14b
expression vector and expressed in two strains of
E. coli. The expression of recombinant Mcp4 (rMcp4)
was highest when using the pET14b::Mcp4a construct
in combination with the E. coli BL21(DE3) pLysS
strain grown for 8 h after induction. Recombinant
macrocypins rMcp1 and rMcp3 were expressed mainly
as insoluble inclusion bodies, and rMcp4 was
expressed as an equal distribution of protein between
the soluble form and inclusion bodies. All three rMcps
were purified fromthe inclusion bodies, which were
almost completely solubilized in 3 m urea. One-step
purification using size-exclusion chromatography
yielded purified recombinant macrocypins rMcp1 and
rMcp4, while rMcp3 still contained some impurities,
which were taken into consideration when calculating
the concentration.
Characterization of macrocypins
Recombinant macrocypins rMcp1, rMcp3 and rMcp4
were resolved on SDS–PAGE under reducing condi-
tions as single 19 kDa bands (Fig. 4A). Under non-
reducing conditions, however, they all showed an
additional band at 38 kDa, corresponding to a
dimer, probably formed between the single cysteines
present in each protein. The calculated isoelectric
point of 5.1 for Mcp4 was confirmed by IEF and
was similar to the isoelectric point ofthe natural
macrocypin isolated from basidiocarps of M. procera.
For Mcp1 and Mcp3, the calculated isoelectric points
were 4.8, which was also confirmed by IEF
(Fig. 4B).
N-terminal sequences were confirmed for all three
recombinant macrocypins. That for rMcp1 [NH
2
-
(M)GFEDG] revealed N-terminal cleavage of methio-
nine in approximately one-third ofthe molecules.
N-terminal sequences of rMcp3 and rMcp4 (NH
2
-
ALEDG) showed complete cleavage of N-terminal
methionine. N-terminal cleavage of methionine in
E. coli is strongly influenced by the amino acid resi-
dues at the P1¢,P2¢ and P3¢ positions (the P1 position
being the first methionine) [15]. In the case of macro-
cypins, the NH
2
-MALE sequence favours N-terminal
methionine cleavage in E. coli, and the NH
2
-MGFE
sequence of rMcp1 favours only partial cleavage.
The far-UV CD spectra of rMcp1 and rMcp4 con-
firmed the expectation fromthe sequences that the
conformations oftheinhibitors are very similar
(Fig. S5A). The marked tryptophan bands, seen also
in clitocypin [9] and ascribed to interaction of buried
tryptophan residues, prevent analysis of secondary
structure, but underline the similarity in tertiary struc-
ture, at least in this region, as well as of secondary
structure.
Clitocypin has been proven to be a very stable pro-
tein [5,9]. The temperature and pH stability of recom-
binant macrocypins were determined by following their
inhibitory activity (measured after return to native
conditions) after heating and after incubation at
extremes of pH. The macrocypins rMcp1 and rMcp3
retained their inhibitory activity after heating at 75 °C,
or even at 100 °C, for 15 min, whereas rMcp4 partially
lost its inhibitory activity after heating at 75 °C for
15 min and completely lost its inhibitory activity after
AB
Fig. 4. Comparison of natural and recombinant macrocypins by
SDS–PAGE (A) and IEF (B). Purified natural (nMcp) and recombinant
macrocypins (rMcp) were subjected to SDS–PAGE analysis under
reducing denaturing conditions and to IEF. Lane M, protein mole-
cular mass markers; lane S, standard protein IEF markers; lane 1,
natural macrocypin (nMcp); lane 2, recombinant macrocypin 4
(rMcp4); lane 3, recombinant macrocypin 1 (rMcp1); lane 4, recom-
binant macrocypin 3 (rMcp3).
Fungal cysteineproteaseinhibitors J. Sabotic
ˇ
et al.
4338 FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS
heating at 100 °C. Similarly, rMcp1 and rMcp3
retained their inhibitory activities after incubation in
acidic (pH 2) or alkaline (pH 11) conditions. While
rMcp4 lost its inhibitory activity after incubation at
pH 2, incubation at pH 11 had no influence.
Stability was also examined by following conforma-
tion directly by CD. rMcp1 and rMcp4 were unfolded
on thermal denaturation, with closely similar transi-
tions, with temperature midpoints of 78 °C (Fig. S5B).
The similarity of this value to that for clitocypin shows
that the differences in sequence between these three
inhibitors are not critical for the stability ofthe pro-
teins. Combined, the above results show that the inhib-
itors unfold reversibly. Measurements of CD spectra at
pH 2.2 and pH 11 showed only a slight decrease in
ellipticity after 24 h of exposure.
Specificity of macrocypins
The inhibitory specificities ofthe natural macrocypin
isolated from basidiocarps and the three recombinant
macrocypins were determined against several cysteine
proteases. Association (k
a
) and dissociation (k
d
) rate
constants and equilibrium constants (K
i
) were deter-
mined by continuous assays for papain, cathepsins L
and V, and legumain (Table 1), for which typical
biphasic progress curves were obtained. For inhibition
of cathepsins S, K, B and H and trypsin by macrocy-
pins, only equilibrium constants were determined
(Table 2). Macrocypins 1 and 3 were found to be effec-
tive inhibitorsof papain, cathepsin L and cathepsin V,
with a mean K
i
value of 0.5 nm. Macrocypin 4 was
also an effective inhibitor of papain but exhibited
weaker inhibition of cathepsin L and V than the other
two recombinant macrocypins. The sample of natural
macrocypin showed weaker inhibition for these
Table 1. Inhibition ofcysteine proteases by natural and recombi-
nant macrocypins. Kinetic and equilibrium constants for the inhibi-
tion of papain, cathepsins L and V, and legumain were determined
under pseudo-first-order conditions in continuous kinetic assays at
25 °C and calculated by nonlinear regression analysis according to
Morrison [32]. Standard deviation is given where appropriate; ND,
not determined; nMcp, natural macrocypin; rMcp1, recombinant
macrocypin 1; rMcp3, recombinant macrocypin 3; rMcp4, recombi-
nant macrocypin 4.
Enzyme 10
)6
k
a
(M
)1
Æs
)1
)10
4
k
d
(s
)1
) K
i
(nM)
nMcp
Papain 0.36 ± 0.07 18.3 ± 3.91 5.04 ± 0.98
Cathepsin L 0.33 ± 0.11 1.25 ± 0.26 3.81 ± 1.66
Cathepsin V 0.08 ± 0.01 9.85 ± 1.54 12.6 ± 3.8
Legumain 0.006 ± 0.001 6.49 ± 0.99 110 ± 23
rMcp1
Papain 2.25 ± 0.49 21.4 ± 0.7 0.95 ± 0.33
Cathepsin L 5.52 ± 0.51 35.1 ± 3.2 0.64 ± 0.22
Cathepsin V 1.48 ± 0.01 10.3 ± 0.7 0.69 ± 0.06
Legumain 0.22 ± 0.04 7.66 ± 4.21 3.38 ± 1.44
rMcp3
Papain 4.28 ± 0.95 5.10 ± 0.81 0.12 ± 0.05
Cathepsin L 3.58 ± 0.45 11.1 ± 0.5 0.31 ± 0.06
Cathepsin V 1.88 ± 0.09 8.43 ± 0.76 0.45 ± 0.01
Legumain 0.063 ± 0.020 5.77 ± 1.27 9.17 ± 1.09
rMcp4
Papain 3.41 ± 0.15 6.32 ± 0.75 0.19 ± 0.01
Cathepsin L 1.62 ± 0.55 45.1 ± 5.1 2.76 ± 0.92
Cathepsin V 2.29 ± 0.66 33.3 ± 6.3 1.44 ± 0.11
Legumain ND ND > 1000
Table 2. Inhibition of various proteases by natural and recombinant mycocypins. Equilibrium constants for the inhibition of different prote-
ases were determined in continuous or stopped kinetic assays and analyzed according to Morrison [32] or Henderson [33], respectively.
Kinetic data for the interaction of clitocypin with papain, cathepsins L, K and H, and legumain were reported previously [6]. Standard devia-
tion is given where appropriate. nMcp, natural macrocypin; rMcp1, recombinant macrocypin 1; rMcp3, recombinant macrocypin 3; rMcp4,
recombinant macrocypin 4; nClt, natural clitocypin; rClt, recombinant clitocypin; n.i., no inhibition.
Enzyme
K
i
(nM)
nMcp rMcp1 rMcp3 rMcp4 nClt rClt
Papain 5.04 ± 0.98 0.95 ± 0.33 0.12 ± 0.05 0.19 ± 0.01 2.5 ± 0.94 6.2 ± 0.55
Cathepsin L 3.81 ± 1.66 0.64 ± 0.22 0.31 ± 0.06 2.76 ± 0.92 0.03 ± 0.002 0.02 ± 0.001
Cathepsin V 12.6 ± 3.77 0.69 ± 0.06 0.45 ± 0.01 1.44 ± 0.11 0.14 ± 0.01 0.08 ± 0.03
Cathepsin S 47.1 ± 3.1 23.1 ± 1.2 5.1 ± 0.5 6.3 ± 0.6 3.2 ± 0.3 2.2 ± 0.3
Cathepsin K 4.5 ± 0.5 170 ± 20 17.5 ± 1.2 21.8 ± 5.2 0.02 ± 0.005 0.03 ± 0.002
Cathepsin B 515 ± 36 490 ± 18 > 1000 125 ± 10 > 1000 > 1000
Cathepsin H 370 ± 11 100 ± 10 24 ± 5 32 ± 6 n.i. n.i.
Legumain 110 ± 23 3.38 ± 1.44 9.17 ± 1.09 > 1000 7.1 ± 1.12 21.5 ± 2.81
Trypsin n.i. n.i. n.i. 160 ± 14 n.i. n.i.
Pepsin n.i. n.i. n.i. n.i. n.i. n.i.
J. Sabotic
ˇ
et al. Fungal cysteineprotease inhibitors
FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS 4339
enzymes than the recombinant macrocypins. Inhibition
of cathepsins S and K by recombinant macrocypins
was somewhat weaker, with K
i
values in the range of
5–25 nm, and 10 times higher for inhibition of cathep-
sin K by rMcp1. Cathepsin B, which has both endo-
peptidase and exopeptidase activities, was inhibited by
macrocypins with K
i
values in the micromolar range,
with the exception of rMcp3 (K
i
>1lm). By contrast,
cathepsin H was inhibited by natural macrocypin and
rMcp1, with K
i
values in the micromolar range, while
rMcp3 and rMcp4 inhibited with 10-fold lower values.
Like clitocypin, recombinant macrocypins inhibited the
cysteine protease legumain, a member ofthe C13 fam-
ily, with an average K
i
value of 6 nm. The natural
macrocypin exhibited only very weak inhibition of
legumain (K
i
in the micromolar range), while rMcp4
showed no inhibition at all. The serine protease trypsin
was not inhibited by natural macrocypin, rMcp1 or
rMcp3, while rMcp4 exhibited weak inhibition with a
K
i
value in the micromolar range. The aspartic prote-
ase pepsin was not inhibited by natural or recombinant
macrocypins.
The ability of natural and recombinant clitocypins
[6] to inhibit cathepsins V, S and B was also deter-
mined for comparison (Table 2). Clitocypin is an effec-
tive inhibitor of cathepsins V and S. The weak
inhibition of cathepsin B reported for the natural clito-
cypin, with a K
i
value of 0.48 lm [5], was not con-
firmed with either recombinant or natural clitocypin,
for which K
i
values were > 1 lm.
Discussion
A novel cysteineprotease inhibitor, macrocypin, has
been isolated from basidiocarps ofthe parasol mush-
room (M. procera), in addition to a putative clito-
cypin-like cysteineprotease inhibitor. Based on
similarities in genetic and biochemical characteristics,
macrocypin was assigned to the mycocypin family of
fungal cysteineprotease inhibitors, family I48 in the
merops database, together with clitocypin from
clouded agaric (C. nebularis) [6,7].
Based on the partial protein sequence, several macr-
ocypin-coding genes and corresponding cDNAs were
amplified and sequenced, together with the promoter
and 5¢ UTR and 3¢UTR sequences (Fig. S3). The
diversity observed was even greater than that observed
for clitocypin-coding genes [7], the macrocypin
sequences being divided into five groups. The variabil-
ity was distributed throughout the coding sequence
and comprised one to five consecutive amino acid sub-
stitutions (Fig. 2). The variability was not limited to
the coding sequence, as two different promoter
sequences were cloned. A few 3¢ UTR sequences were
found that showed no sequence diversity, but differed
in their length. Different promoter and 5¢UTR and
3¢UTR sequences, and their lengths, together with
some differences found in intron sequences and their
lengths, which could influence transcription, splicing,
mRNA transport, stability and translation, all suggest
complex regulation of macrocypin expression at diff-
erent levels.
Macrocypin- and clitocypin deduced amino acid
sequences show similarities, despite a low overall
sequence identity of 17–21% (Fig. 3). They both have
high contents of proline and tyrosine and low contents
of leucine. A major difference between clitocypin and
macrocypin sequences lies in the presence of sulfur-
containing amino acids in macrocypins, but not in
clitocypins. In spite of very low overall sequence simi-
larity, several amino acid residues are conserved in all
macrocypin and clitocypin sequences, mainly in the
N-terminal half (Fig. 3). These are probably important
for the inhibitory activity and⁄ or structure, and many
of them are proline residues.
A similarity search using macrocypin deduced amino
acid sequences against the translated nucleotide data-
base at the NCBI server showed significant similarity
to the putative L. bicolor clitocypin-like cysteine prote-
ase inhibitor. Alignment ofthe deduced sequences of
the latter with those of macrocypin from M. procera
and with clitocypin from C. nebularis revealed con-
served amino acid residues (Fig. S6), the majority of
which were already present in the alignment of macro-
cypin and clitocypin deduced amino acid sequences,
confirming their functional and ⁄ or structural imp-
ortance.
Macrocypins and clitocypins exhibit similar basic
biochemical characteristics. They have similar molecu-
lar masses of 19 and 16.8 kDa and similar isoelectric
points of around 4.8. They both exhibit stability
against high temperature and extremes of pH. The CD
spectrum in the far-UV region for macrocypin, show-
ing the characteristic peak around 232 nm that indi-
cates an unusually strong contribution of tryptophan
residues (Fig. S5A), indicates further structural similar-
ity to clitocypin [6,9].
The high degree of diversity in macrocypin gene
sequences indicates a mixture ofinhibitors in the natu-
ral macrocypin sample isolated from basidiocarps of
M. procera. In order therefore to characterize the
inhibitors further, recombinant macrocypins were pre-
pared. Three different macrocypin cDNA clones were
used that belong to different macrocypin groups or
isoforms. Heterologous expression in the bacterial
expression system proved successful for all three,
Fungal cysteineproteaseinhibitors J. Sabotic
ˇ
et al.
4340 FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS
inhibitory macrocypins (rMcp1, rMcp3, rMcp4) being
obtained by one-step purification from inclusion bodies
with high yields of 50–100 mgÆL
)1
.
The inhibitory profiles of macrocypins and clito-
cypin for several cysteine proteases are similar, but not
identical. Ofthecysteine proteases tested, macrocypins
inhibit papain and cathepsins L and V most strongly.
Compared with clitocypin [6], macrocypins are stron-
ger inhibitorsof papain, as a result of higher rate
constants of association, but weaker inhibitors of
cathepsin L, mainly because of increased rate constants
of dissociation. Cathepsins S and K are inhibited by
macrocypins with K
i
values in the nanomolar range,
while clitocypin inhibits cathepsin K with K
i
values in
the picomolar range. The most notable difference
between macrocypin- and clitocypin-inhibition profiles
for cysteine proteases is the weak inhibition by macro-
cypins of cathepsins B and H, the papain-like prote-
ases with endopeptidase and exopeptidase activities. As
with clitocypin, legumain, a member of C13 family, is
inhibited by Mcp1 and Mcp3 with K
i
values in the
micromolar range. The inhibition profile of rMcp4,
with K
i
>1lm for legumain inhibition and K
i
values
in the nanomolar range for papain-like proteases, con-
trasts with those of other macrocypins that inhibit
both papain-like proteases and legumain with K
i
values
in the same range. This strongly suggests different
binding sites for the inhibition ofthe two families of
cysteine proteases. Similarly, two independent and
nonoverlapping binding sites have been reported for
family C1 and C13 inhibition by legumain-inhibiting
cystatins C, E ⁄ M and F [16].
The ability of macrocypins to inhibit proteases of
other catalytic classes was tested. Neither macrocypins
nor clitocypin [5] inhibit the aspartic protease pepsin.
The serine protease trypsin is weakly inhibited by
rMcp4, which is the most significant difference in the
inhibitory profiles of macrocypins and clitocypin.
The physiological function ofthe macrocypin cyste-
ine protease inhibitor family is proposed to be defence
against pathogen infection and ⁄ or predation by insects
or other pests, analogously to the phytocystatins that
are involved in plant defence by inhibiting exogenous
cysteine proteases during herbivory or infection [17].
The sequence diversity includes amino acid sites of
positive selection. The variations in inhibitory profile
between different members ofthe macrocypin family
reveal different specificities and strengths of inhibition
of cysteine proteases of different evolutionary families,
and even a serine protease. These findings together
suggest an adaptation process and the selection of
appropriate inhibitor isoforms providing effective
defence. In addition, a regulatory role in intracellular
proteolysis may also be considered for mycocypins,
because cysteineprotease activity is present in basidio-
mycetes and its inhibition by clitocypin was shown in
a few selected basidiomycete species belonging to dif-
ferent orders [8].
In conclusion, we have characterized a novel family
of fungal cysteineproteaseinhibitors – the macrocy-
pins – from M. procera, at the genetic and biochemical
levels and analyzed their inhibition profiles. Similarity
to clitocypin from C. nebularis is evident at all these
levels, suggesting that they belong to the same family
of cysteineprotease inhibitors, the mycocypins, thus
substantiating the establishment ofthe I48 family of
protease inhibitors in the MEROPS classification that
previously comprised only one member. In addition to
the high conformational stability of mycocypins, their
other common characteristic is high genetic diversity,
with sequence variability influencing the inhibitory
activity in macrocypins, but not in clitocypins. Myco-
cypins could find use in medical research, as their
unique inhibitory profiles could answer the challenge
of finding highly selective inhibitors against proteases
important in certain stages of diseases, without affect-
ing nontarget proteases. Additionally, certain represen-
tatives ofthe macrocypin family, showing inhibition of
different classes of proteases, would have applications
in plant protection. Double-inhibitory activity against
two catalytic classes of proteases in one stable mole-
cule could provide more effective protection of plants
against insect pests.
Experimental procedures
Isolation ofcysteineproteaseinhibitors from
M. procera
Basidiocarps ofthebasidiomycete M. procera were col-
lected from their natural habitat and frozen at )20 °C.
Thawed basidiocarps were homogenized in an equal volume
of 0.1 m Tris–HCl buffer, pH 7.5, containing 0.5 m NaCl,
and centrifuged at 8000 g for 30 min. Ammonium sulfate
was added to the supernatant to a final concentration of
1.3 m before application to a column of Phenyl Sepharose
(GE Healthcare, Uppsala, Sweden). After thorough wash-
ing with 0.1 m Tris–HCl buffer, pH 7.5, containing 1.3 m
ammonium sulphate, the bound proteins were eluted by a
1.3–0 m gradient of ammonium sulphate in the same buffer.
Inhibitory fractions, measured against papain, were pooled,
concentrated by ultrafiltration (Amicon UM-10; Millipore,
Vienna, Austria) and dialyzed against 0.02 m Tris–HCl, pH
7.5. The sample was then applied to a column of DEAE–
Sephacel (Pharmacia-LKB, Uppsala, Sweden) equilibrated
with 0.02 m Tris–HCl, pH 7.5. Bound proteins were eluted
J. Sabotic
ˇ
et al. Fungal cysteineprotease inhibitors
FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS 4341
with a gradient of 0–0.4 m NaCl in the same buffer. Inhibi-
tory fractions were pooled and subjected to an affinity col-
umn of carboxymethylpapain–Sepharose, prepared as
described previously [5], and equilibrated with 0.02 m Tris–
HCl, pH 7.5, containing 0.3 m NaCl. Bound inhibitory
fractions were eluted with 0.02 m NaOH, neutralized with
dilute HCl, and pooled and concentrated by ultrafiltration
(Amicon UM-3).
N-terminal sequence analysis
Automated amino acid sequencing of purified natural and
recombinant macrocypins was performed as described pre-
viously [6]. An internal peptide sequence was determined
after cleavage with cyanogen bromide in 80 % formic acid
at room temperature in the dark for 36 h. The resulting
peptide fragments were separated using reverse-phase
HPLC, as described previously [6].
Isolation of genomic DNA and total RNA
Basidiocarps ofthebasidiomycete M. procera, harvested
from their natural habitat, were frozen in liquid nitrogen,
homogenized and stored at )80 °C until use. High-
molecular-weight genomic DNA was isolated from frozen
powdered tissue as described previously [18] and total
RNA was extracted using an RNeasy Kit (Qiagen,
Vienna, Austria) according to the manufacturer’s protocol
for isolation of total RNA from plant tissues and fila-
mentous fungi.
Cloning ofthe genomic and cDNA sequences
encoding macrocypins
First-strand cDNA was synthesized fromthe total RNA by
RT-PCR using a GeneAmp RNA PCR Core Kit (Applied
Biosystems, Foster City, CA, USA) with anchored oli-
go(dT)-adapter primer (dT
(17)
3¢RACE) (Table S1). Forward
and reverse degenerate primers (forward 1N-mar-Clit,
nested forward 2N-mar-Clit and reverse C-mar-Clit) were
designed based on the N-terminal amino acid sequence and
an internal peptide fragment sequence. First-strand cDNA
was used for PCR to amplify the partial macrocypin cDNA
sequence, which was then used to design specific primers.
Forward specific primer (Mp-CliHom-N-uni) was used to
amplify the 3¢ end ofthe cDNA sequence, using the 3¢
RACE method, together with the 3¢RACE adapter primer.
The resulting PCR product was used in a secondary PCR
with two different nested forward primers (Mp-CliHom-N-
A12 and Mp-CliHom-N-A3), together with the 3¢ RACE
adapter primer.
To amplify the complete macrocypin gene (mcp) with its
upstream and downstream regions, Genome Walker
libraries were constructed using the Genome WalkerÔ
Universal kit (BD Biosciences Clontech) according to the
manufacturer’s instructions. High-molecular-weight geno-
mic DNA (2.5 lg) was digested separately with two restric-
tion enzymes (PvuII and StuI) at 37 °C overnight and after
purification by ethanol precipitation, Genome WalkerÔ
Adaptors were ligated to the digested DNA at 16 °C over-
night. The resulting Genome Walker libraries were used as
templates in genome walking PCR amplifications, using
nested forward specific primers (Mp-CliHom-ter1A and 1)
for downstream amplification and nested reverse specific
primers (Mp-CliHom-pro 1 and 2) for upstream amplifica-
tion, paired with Adaptor Primer 1 and Nested Adaptor
Primer 2 provided by the manufacturer. Advantage 2 Poly-
merase Mix (Clontech) was used for amplification under
the conditions suggested by the manufacturer.
Complete mcp gene and cDNA sequences were obtained
using pairs of primers annealing to the 5¢ UTR (Mcp-N-
A12-1 and Mcp-N-A3-1 with nested primers Mcp-N-uni-1
or Mp-CliHom-N-uni) and the 3¢ UTR (Mcp-C-uni-1 with
nested primers Mp-CliHom-C-uni, Mp-CliHom-C-A12 or
Mp-CliHom-C-A3) regions in two-step PCR amplification,
using nested primers in the secondary PCR with recombi-
nant Taq polymerase (MBI Fermentas, Vilnius, Lithuania).
All PCR products were cloned into the pGEM-T Easy
Vector System (Promega, Vienna, Austria) for sequencing
by the Automated DNA Sequencing Service at MWG
Biotech (Ebersberg, Germany).
Sequence analyses
Sequence analysis and multiple sequence alignments were
performed in the BioEdit Sequence Alignment Editor
(http://www.mbio.ncsu.edu/bioedit/bioedit.html). Promoter
analysis was performed using the Transcription Element
Search System (TESS, [19]; http://www.cbil.upenn.edu/cgi-
bin/tess/tess). Similarity searches were performed using
blastn and tblastn algorithms [13] against different data-
bases at the NCBI (http://www.ncbi.nlm.nih.gov/BLAST).
Evolutionary analysis
The Datamonkey web interface [20] (http://www.datamon-
key.org) was used to examine selective pressure acting upon
individual sites of codon alignments. Three methods were
implemented to test for purifying or diversifying selection:
the single likelihood ancestor counting (SLAC); fixed effects
likelihood (FEL); and random effects likelihood (REL)
[21]. A P-value of 0.05 was used for inference of positive
and negative selection for individual codons. A hierarchical
and information theoretic model selection procedure was
applied to choose a model of nucleotide substitution.
HKY85 was selected as the optimal time-reversible nucleo-
tide substitution model using the implementation in the
HyPhy package [22].
Fungal cysteineproteaseinhibitors J. Sabotic
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et al.
4342 FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS
Expression and purification of recombinant
macrocypins
Whole-length cDNA clones of Mcp1a and Mcp3a were
used as templates in the PCR amplification with Pfu DNA
polymerase (Promega) and primers that introduced NdeI
and BamHI restriction sites to the 5¢ and 3¢ ends of the
insert, respectively. After resequencing the resulting prod-
uct, and digesting the inserts and vectors with NdeI ⁄ BamHI
(New England Biolabs, Frankfurt am Main, Germany), the
inserts were subcloned into pET3a and pET11a vectors
(Novagen) to generate recombinant proteins without tags.
Similarly, NcoI and NdeI restriction sites were introduced
into the 5¢ and 3¢ ends ofthe whole-length cDNA of
Mcp4a. After digestion ofthe Mcp4a insert and vector with
NcoI ⁄ NdeI (New England Biolabs), the insert was subcl-
oned into the pET14b expression vector (Novagen) to gen-
erate protein without tags. All constructed expression
vectors with inserts were transformed into E. coli
BL21(DE3), which was grown in LB (Luria–Bertani) med-
ium supplemented with 100 lgÆmL
)1
of ampicillin at 37 °C.
The construct pET14b::Mcp4a was also transformed into
the E. coli BL21(DE3) pLysS strain, which was grown at
37 °C in LB medium supplemented with 100 lgÆmL
)1
of
ampicillin and 34 lgÆmL
)1
of chloramphenicol. When the
attenuance (D) at 600 nm reached 1–1.2, the inducer iso-
propyl thio-b-d-galactoside was added to a final concentra-
tion of 0.4 mm for strains transformed with pET3a or
pET14b constructs and to a final concentration of 1 mm
for strains transformed with the pET11a construct. Cells
were then grown for an additional 6 or 8 h. They were har-
vested by centrifugation for 15 min at 6000 g, resuspended
in buffer A (50 mm Tris–HCl, pH 7.5, 0.1 % Triton X-100,
2mm EDTA), frozen and thawed once, then sonicated at
4 °C. The insoluble fraction was separated by centrifuga-
tion for 15 min at 10000 g, redissolved in the same buffer
containing 3 m urea and solubilized by stirring for 4 h at
4 °C. The remaining insoluble material was removed by
centrifugation and the supernatant was applied to a Sepha-
rose S200 column (4 · 110 cm) equilibrated with Tris–HCl
buffer, pH 7.5, containing 0.3 m NaCl. Inhibitory fractions
were pooled and concentrated by ultrafiltration (Amicon
UM-3) to approximately 1 mgÆmL
)1
.
SDS–PAGE and IEF
Proteins were separated by 12.5% SDS–PAGE under dena-
turing and reducing or non-reducing conditions, as appro-
priate, and stained using Coomassie Brilliant Blue. The
molecular mass values ofthe separated proteins were
estimated using low-molecular-mass standard proteins of
14.4–97 kDa (LMW Calibration Kit; GE Healthcare). The
Phast System (Pharmacia) was used to perform SDS–
PAGE (precast 8–25 % gradient gels) and IEF (precast pH
3–9 gradient gels), as described previously [6]. Theoretical
molecular mass and pI values were determined from
sequences using the protparam tool available at the Exp-
aSy server ofthe Swiss Institute of Bioinformatics (http://
www.expasy.org/tools/protparam.html).
Inhibition assay
Inhibitory activities against papain were determined as
described previously [5] using Bz-DL-Arg-2-naphthylamide
(Sigma, Taufkirchen, Germany) as the substrate [23].
Enzymes and determination of kinetic constants
Human cathepsin H (EC 3.4.22.16) and cathepsin L (EC
3.4.22.15) were purified as described previously [24]. Papain
(2· crystallized) (EC 3.4.22.2) was further purified by affin-
ity chromatography [25]. Beta-trypsin (EC 3.4.21.4) was
prepared from type IX trypsin (Sigma), as described previ-
ously [26]. Legumain (EC 3.4.22.34) was isolated from pig
kidney cortex following a previously described procedure
[27]. Recombinant human cathepsin K (EC 3.4.22.38) [28],
cathepsin S (EC 3.4.22.27) [29] and cathepsin B (EC
3.4.22.1) [30], all expressed in E. coli, were provided by
Prof. Boris Turk, and recombinant human cathepsin V (EC
3.4.22.43) [31] was provided by Professor Dus
ˇ
an Turk
(both fromthe Department of Biochemistry and Molecular
and Structural Biology, Jozˇ ef Stefan Institute, Ljubljana,
Slovenia).
Inhibition kinetics for natural and recombinant macro-
cypins and clitocypins were measured under pseudo-first-
order conditions, as previously described [6]. Continuous
kinetic assays were performed for thecysteine proteases
papain, cathepsin L and cathepsin V using benzyloxycar-
bonyl (Z)-Phe-Arg-7-amido-4-methylcoumarin (AMC) as
substrate, and for legumain with Z-Ala-Ala-Asn-AMC as
the substrate, while stopped assays were performed for
cathepsins K, S and B using Z-Phe-Arg-AMC as the sub-
strate and for cathepsin H with Arg-AMC as the substrate
[6]. Trypsin was assayed using the stopped kinetic assay
with fluorogenic substrate Z-Phe-Arg-AMC in 0.1 m Tris–
HCl buffer, pH 8.0, containing 1.5 mm EDTA and 0.02 m
CaCl
2
. Data for continuous assays were analyzed by non-
linear regression analysis according to Morrison [32], while
kinetic constants for cathepsins K, S, B and H, and trypsin,
were determined according to Henderson [33]. Porcine
pepsin (3.4.32.1) from Sigma was assayed in 0.1 m acetate
buffer, pH 3.5, using the fluorogenic substrate fluorescein
isothiocarbamoyl–hemoglobin, as described for fluorescein
isothiocarbamoyl–casein [34].
CD spectroscopy
CD spectra measurements and thermal-unfolding transi-
tions were performed on an Aviv model 60 spectropolarim-
J. Sabotic
ˇ
et al. Fungal cysteineprotease inhibitors
FEBS Journal 276 (2009) 4334–4345 ª 2009 The Authors Journal compilation ª 2009 FEBS 4343
[...]... D190–D195 13 Altschul SF, Madden TL, Schaffer AA, Zhang J, Zhang Z, Miller W & Lipman DJ (1997) Gapped BLAST and PSI-BLAST: a new generation of protein database search programs Nucleic Acids Res 25, 3389–3402 14 Martin F, Aerts A, Ahren D, Brun A, Danchin EG, Duchaussoy F, Gibon J, Kohler A, Lindquist E, Pereda V et al (2008) The genome of Laccaria bicolor provides insights into mycorrhizal symbiosis Nature... proteinases Anal Biochem 47, 280–293 24 Popovic T, Puizdar V, Ritonja A & Brzin J (1996) Simultaneous isolation of human kidney cathepsins B, H, L and C and their characterisation J Chromatogr B: Biomed Appl 681, 251–262 25 Blumberg S, Schechter I & Berger A (1970) The purification of papain by affinity chromatography Eur J Biochem 15, 97–102 26 Strop P & Cechova D (1981) Separation of alpha-trypsin and beta-trypsin... ClustalW alignment of partial clitocypin-like gene sequences from M procera (MpClt) with that of clitocypin from C nebularis (CnClt) Fig S3 ClustalW alignment ofthe full-length macrocypin gene with promoter and cDNA sequences Fig S4 Expression and purification of recombinant macrocypins rMcp1 (A) , rMcp3 (B) and rMcp4 (C) Fig S5 Far UV CD spectra and thermal unfolding transitions of recombinant macrocypins... measurements, discussion ofthe results and critical reading ofthe manuscript Dr Dusˇ an Kordisˇ is gratefully acknowledged for assistance in the evolutionary analysis of sequences We thank Adrijana Leonardi for determining N-terminal protein sequences References 1 Turk B, Turk D & Turk V (2000) Lysosomal cysteine proteases: more than scavengers Biochim Biophys Acta 1477, 98–111 2 Turk B (2006) Targeting... enzymes and subcellular particles Fungal cysteineproteaseinhibitors interacting with tightly bound inhibitors Biochem J 127, 321–333 34 Twining SS (1984) Fluorescein isothiocyanate-labeled casein assay for proteolytic enzymes Anal Biochem 143, 30–34 Supporting information The following supplementary material is available: Fig S1 Clitocypin-encoding genes are present in theMacrolepiotaprocera genome... for 2 h at room temperature in 0.1 m citrate buffer, pH 2, in 0.1 m phosphate buffer, pH 6.5, or in 0.1 m Tris–HCl buffer, pH 11, and neutralized afterwards Residual activities were then determined against papain with Z-Phe-Arg-para-nitroanilide as the substrate [5] Acknowledgements This work was supported by the Slovenian Research Agency Grant No P4-0127 (J.K.) We are very grateful to Dr Roger Pain for... Dobersek A, Guncar G & Turk D (2008) Inhibitory fragment fromthe p41 form of invariant chain can regulate activity ofcysteine cathepsins in antigen presentation J Biol Chem 283, 14453–14460 32 Morrison JF (1982) The slow-binding and slow, tightbinding inhibition of enzyme-catalyzed reactions Trends Biochem Sci 7, 102–105 33 Henderson PJF (1972) Linear equation that describes steady-state kinetics of enzymes... rMcp1 and rMcp4 Fig S6 ClustalW alignment of macrocypin and clitocypin sequences with deduced clitocypin-like sequences from Laccaria bicolor genome Table S1 List of degenerate and specific primers used in PCR reactions Doc S1: Supplementary results Doc S2: Supplementary experimental procedures This supplementary material can be found in the online article Please note: As a service to our authors and readers,...ˇ J Sabotic et al Fungal cysteineproteaseinhibitors eter (Aviv, Lakewood, NJ, USA), as described previously [9] Temperature and pH stability Recombinant macrocypins (0.1 mgÆmL)1) were incubated for 15 min in 0.1 m phosphate buffer, pH 6.5, containing 1.5 mm EDTA and 5 mm dithiothreitol, at 37, 75 or 100 °C, then incubated for 1 h at room temperature Macrocypins (0.1 mgÆmL)1) were also incubated for... Purif 15, 213–220 29 Kopitar G, Dolinar M, Strukelj B, Pungercar J & Turk V (1996) Folding and activation of human procathepsin S from inclusion bodies produced in Escherichia coli Eur J Biochem 236, 558–562 30 Kuhelj R, Dolinar M, Pungercar J & Turk V (1995) The preparation of catalytically active human cathepsin B from its precursor expressed in Escherichia coli in the form of inclusion bodies Eur . Macrocypins, a family of cysteine protease inhibitors from
the basidiomycete Macrolepiota procera
Jerica Sabotic
ˇ
1
, Tatjana Popovic
ˇ
1
, Vida Puizdar
2
and. report a novel family of cysteine prote-
ase inhibitors from basidiocarps, or fruiting bodies,
of the basidiomycete Macrolepiota procera, and have
characterized