Improvement of the catalytic properties of penicillin G acylase from Escherichia coli ATCC 11105 by selection of a new substrate specificity

Cloned penicillin G acylase (PGA) from Escherichia coli ATCC 11105 was mutagenized in vivo using N-methyl-N-nitrosoguanidine. Mutants of PGA were selected by their ability to allow growth of the host strain E. coli M8820 with the new substrates phenylacetyl--alanyl-l-proline (PhAc-Ala-Pro) phthalyl-l-leucine (Pht-Leu) or phthalylglycyl-l-proline (Pht-Gly-Pro) as sole source of proline and leucine respectively. PGA mutants were purified and immobilized onto spherical methacrylate (G-gel). The immobilized form of mutant PGA selected with (PhAc-gbAla-Pro) hydrolyzed 95% of 9 mmol penicillin G 30% faster than wild-type PGA using the same specific activities. The specific activity of the soluble enzyme was 2.7-fold, and inhibition by phenylacetic acid was halved. Immobilized PGA mutant selected with Pht-Gly-Pro hydrolyzed penicillin G 20% faster than wild-type PGA. The K _m of the soluble enzyme was increased 1.7-fold. Furthermore, the latter two mutants were also 3.6-fold more stable at 45° C than wild-type PGA. The specific activity of the mutant selected with Pht-Leu was 6.3-fold lower, and inhibition by phenylacetic acid was increased 13-fold.     

Antibacterial Effects of Water-Soluble Low-Molecular-Weight Chitosans on Different Microorganisms

Low-molecular-weight chitosans with a viscosity-average molecular weight (M) of 5 to 27 kDa and an equal degree of deacetylation (DD, 85%) were highly active against Pseudomonas aureofaciens, Enterobacter agglomerans, Bacillus subtilis, and Bifidobacterium bifidum791, causing death in 80 to 100% of cells. An exception to this tendency was Escherichia coli, for which the rate of cell death induced by the 5-kDa chitosan, was 38%. The antibacterial effect was manifested as early as 10 min after the incubation of 12-kDa chitosan with B. subtilis or E. coli cells. Candida krusei was almost insensitive to the above crab chitosans. However, Candida krusei was highly sensitive to chitosans with M 5, 6, 12, 15.7, and 27 kDa: the minimum inhibitory concentration (MIC) varied from 0.06 to 0.005%. Chitosans with M 5, 12, and 15.7 kDa exerted an antibacterial effect on Staphylococcus aureus. Chitosans with M 5, 15.7, and 27 kDa had no effect on Bifidobacterium bifidum ATCC 14893. The antibacterial effect of the 4-kDa chitosan on E. coli and B. bifidum 791 increased with DD in the range 55–85%.     

The effect of the ribosomal protein S1 from Escherichia coli on the synthesis in vitro of bacterial-, DNA phage- and RNA phage proteins.

Summary Using an in vitro preparation for protein synthesis, we have studied the effect of the ribosomal protein S1 fromEscherichia coli on the synthesis of the coat protein of the RNA-containing phages Q and MS2, on that of an early and a ate enzyme encoded by the DNA containing phage T7, and on that of anthranilate synthetase, an enzyme encoded by the bacterial tryptophan operon. Our results indicated that for the synthesis of these five proteins the presence of S1 is required. From these results we conclude that S1 is an essential protein for the translation of bacterial and bacteriophage messenger RNA.     

The host specificity system inEscherichia coli SK

E. coli SK has its own enzyme system providing DNA host specificity which differs from the known types of specificity inE. coli K12 andE. coli B. Modification and restriction are observed when the PBVI or PBV3 phages are transferred fromE. coli SK toE. coli B or K12 (and back).A methylase has been isolated fromE. coli SK cells and partly purified. This methylase catalyzesin vitro transfer of the labelled methyl groups from S-adenosylmethionine (SAM) to DNA of both phage and tissue origin which gives rise to 5-methylcytosine (5MC) and 6-methylaminopurine (6MAP). The methylase preparations isolated from the cells at the stationary growth have proved to be 1.5–1.7 times as active as the enzyme from the cells at the logarithmic growth stage. The extract ofE. coli SK cells infected with the phage S_D cannot methylate DNAin vitro. This fact is due tode novo synthesis of the enzyme which disintegrates SAM down to 5-methylthioadenosine (5MTA) and homoserine (HS). This enzyme is not found in the cells infected with the S_D phage in the presence of chloroamphenicole. The activity of the enzyme which disintegrates SAM is the highest between the 4th and the 5th minutes of infection. Thus it may be assumed that this enzyme, most probably, is an early virus specific protein and preventsin vivo methylation of the phage DNA.     

The transport of class I major histocompatibility complex antigens is determined by sequences in the α1 and α2 protein domains

The transport of human-mouse hybrid class I histocompatibility antigens has been studied in a mutant human cell line, 174 × CEM.T2 (T2). T2, a somatic cell hybrid of human B- and T-lymphoblastoid cell lines (B-LCL and T-LCL, respectively), synthesizes HLA-A2 and HLA-B5 glycoproteins, but expresses only low levels of A2 and undetectable levels of B5 at the cell surface. We have previously shown that the products of human class I genes introduced into T2 by transfection behave like the endogenous HLA-B5 glycoproteins, while the products of mouse class I alleles similarly introduced are transported normally to the cell surface. We have now determined that the surface expression of class I glycoproteins in T2 depends on the origin of the ₁ and ₂ domains. Human (HLA-B7) and mouse (H-2D ^p ) hybrid class I genes, encoding the leader, ₁, and ₂ sequences of one species fused to the ₃, transmembrane, and cytoplasmic domains of the other, were transfected into T2. Normal surface expression of the hybrid class I molecule was observed in T2 only when the leader, ₁, and ₂-encoding exons were derived from the mouse gene. The reciprocal construct, encoding human leader, ₁, and ₂ domains fused to the mouse ₃, transmembrane, and cytoplasmic regions, resulted in biosynthesis of a hybrid glycoprotein which was not transported to the cell surface. The products of both constructs were expressed normally in control cells. The effects of glycosylation on class I antigen transport were also studied using mutant class I constructs with altered glycosylation sites. Two mutant B7 genes encoding either an extra glycosylation site at position 176 or no glycosylation sites were transfected into T2. These mutant products were expressed at the cell surface in control cells, but were synthesized and not surface-expressed in T2. These data demonstrate that the HLA/H-2 transport dichotomy in T2 is a function of the origin of the ₁ and/or ₂ domains of the class I glycoprotein, and is not a reflection of glycosylation differences between the human and mouse molecules. Offprint requests to: P. Cresswell.     

The influence of temperature on glucose-6-phosphate dehydrogenase and 6-phosphogluconate dehydrogenase and the regulation of these enzymes in a mesophilic and a thermophilic cyanobacterium

The activities and kinetics of the enzymes G6PDH (glucose-6-phosphate dehydrogenase) and 6PGDH (6-phosphogluconate dehydrogenase) from the mesophilic cyanobacterium Synechococcus 6307 and the thermophilic cyanobacterium Synechococcus 6716 are studied in relation to temperature. In Synechococcus 6307 the apparent K _m's are for G6PDH: 80M (substrate) and 20M (NADP⁺); for 6PGDH: 90M (substrate) and 25M (NADP⁺). In Synechococcus 6716 the apparent K _m's are for G6PDH: 550M (substrate) and 30M (NADP⁺); for 6PGDH: 40M (substrate) and 10M (NADP⁺). None of the K _m's is influenced by the growth temperature and only the K _m's of G6PDH for G6P are influenced by the assay temperature in both organisms. The idea that, in general, thermophilic enzymes possess a lower affinity for their substrates and co-enzymes than mesophilic enzymes is challenged.Although ATP, ribulose-1,5-bisphosphate, NADPH and pH can all influence the activities of G6PDH and 6PGDH to a certain extent (without any difference between the mesophilic and the thermophilic strain), they cannot be responsible for the total deactivation of the enzyme activities observed in the light, thus blocking the pentose phosphate pathway.Abbreviations G6PDH glucose-6-phosphate, dehydrogenase - 6PGDH 6-phosphogluconate dehydrogenase - G6P glucose-6-phosphate - 6PG 6-phosphogluconate - RUDP ribulose-1,5-bisphosphate - Tricine N-Tris (hydroxymethyl)-methylglycine     

Metabolism of a phenylcoumaran substructure lignin model compound in ligninolytic cultures of Phanerochaete chrysosporium

The degradation of the phenylcoumaran substructure model compound methyl dehydrodiconiferyl alcohol by the white-rot wood decay fungus Phanerochaete chrysosporium was investigated using culture conditions optimized for lignin oxidation. Initial attack was in the cinnamyl alcohol side chain, which was oxidized to a glycerol structure. This was subsequently converted by loss of the two terminal carbon atoms, C and C, to yield a C-aldehyde structure, which was further oxidized to the C-acid compound. The next detected intermediate, a phenylcoumarone, was produced by double bond formation between C and C, and oxidation of the C-alcohol to an aldehyde group. Further oxidation of C to an acid yielded the next intermediate. The final identified degradation product was veratric acid. No products from the 5-substituted aromatic ring, and no phenolic products, were found. The initial glycerol-containing intermediate was a mixture of the threo and erythro forms, and no optical activity could be found, suggesting that its formation might have involved nonstereospecific C-C epoxidation followed by non-enzymatic hydrolysis of the epoxide.Abbreviations TLC thin layer chromatography - LDA lithium diisopropyl amide - DDQ 2,3-dichloro-5,6-dicyanobenzoquinone - MS mass spectrometry - UV ultraviolet spectroscopy     

An alpha-L-fucosidase from Thermus sp. with unusually broad specificity

An -L-fucosidase (E.C. 3.2.1.51) exhibiting a wide aglycon specificity expressed in ability of cleaving 1 6-, 1 3-, 1 4-, and 1 2-O-fucosyl bonds in fucosylated oligosaccharides, has been isolated from culture filtrate of Thermus sp. strain Y5. The -L-fucosidase hydrolyzes p-nitrophenyl -L-fucopyranoside with V _max of 12.0 ± 0.1 M/min/mg and K _m = 0.20 ± 0.05 mM and is able to cleave off about 90% of total L-fucose from pronase-treated fractions of fucosyl-containing glycoproteins and about 30% from the native glycoproteins. The purified enzyme is a tetramer with a molecular mass of 240 ± 10 kDa consisting of four identical subunits with a molecular mass of 61.0 ± 0.5 kDa. The N-terminal sequence showed homology to some -L-fucosidases from microbial and plant sources. Hydrolysis of p-nitrophenyl -L-fucopyranoside occurs with retention of the anomeric configuration. Transglycosylating activity of the -L-fucosidase was demonstrated in reactions with such acceptors as alcohols, N-acetylglucosamine and N-acetylgalactosamine while no transglycosylation products were observed in the reaction with p-nitrophenyl -L-fucopyranoside. The enzyme can be classified in glycosyl hydrolase family 29.     

Cohesive single-stranded ends of Streptomyces temperate bacteriophage R4.

Summary The cohesive single-stranded termini of temperate Streptomyces phage R4 were found to be complementary 11 base single-stranded 3-extended DNAs with the sequence: 5-CGCCGTGTCTT-3 3-GCGGCACAGAA-5     

Zur Pigmentarchitektonik der Großhirnrinde des Menschen

Zusammenfassung Mit Hilfe einer neu entwickelten Methode zur Darstellung der Neurolipofuscine werden die am Aufbau der Regio entorhinalis beteiligten Zellschichten elektiv hervorgehoben. Bei einem solchen Vorgehen werden die Unterschiede zwischen den einzelnen Zellarten stärker betont als im Nisslbild, weil nur eine Cytoplasmakomponente dargestellt wird. Diese Beschränkung erlaubt zugleich die Verwendung sehr dicker Schnitte (bis zu 800 ), die — aufgehellt — unter dem Stereomikroskop analysiert werden. Auf diese Weise lassen sich Verfugungen aneinandergrenzender Rindenregionen und Kantenbildungen einzelner Rindenschichten sicher erfassen.Die Schichten des Allocortex unterscheiden sich im Pigmentbild deutlich von denen des Isocortex. Sie gehen nicht kontinuierlich ineinander über. Die Rinde der Regio entorhinalis läßt sich in eine Lamina principalis externa (Pre) und eine Lamina principalis interna (Pri) gliedern. Die äußere und innere Hauptschicht sind meist durch einen zellarmen Faserstreifen (Lamina dissecans) voneinander getrennt. Beide Schichten lassen sich weiter unterteilen (Pre- Pre-, Pre-, Pri-, Pri-, Pri-).In der Regio entorhinalis des Menschen werden 16 Felder pigmentarchitektonisch voneinander unterschieden. Davon bestehen 11 Felder ausschließlich aus allocorticalen Schichten, während die restlichen Areae, welche den Übergang zum Isocortex bilden, aus einer wechselnden Zahl allo- und isocorticaler Zellschichten zusammengesetzt sind.Im Bereich des Gyrus parahippocampalis lassen sich 7 rein allocorticale Felder voneinander abgrenzen. Die Areae gruppieren sich ringartig mit stufenweise abnehmender Organisationshöhe um ein hoch differenziertes Zentrum, das im oralen und lateralen Bezirk der Regio entorhinalis liegt. Das kennzeichnende Merkmal für die zentralen Felder ist eine Aufspaltung von Pri- in drei Schichten (Pri-, Pri-, Pri-). In dem Feld e _{centr. lat.} sind alle drei Unterschichten der Lamina principalis externa enthalten, während in e _{centr. med.} Pre- fehlt. Die angrenzenden Felder mit einheitlichem Pri- lassen sich wieder in Arae mit Pre- (e _{interpol.lat.} , e _caud. ) und ein Gebiet ohne Pre- (e _{interpol. med.} ) gliedern. In den rostralen und medialen Abschnitten verschmelzen Pri- und Pri- zu einer einheitlichen Zellschicht und bilden damit das Feld e _oral. . An der Grenze zum Gyrus ambiens in Nähe des Sulcus rhinencephali inferior findet sich ein schmaler Rindenstreifen, in dem die Schichten der Lamina principalis externa nur mangelhaft ausgebildet sind. Diese limitrophe Zone setzt sich nach caudal in das Grenzfeld zum Praesubiculum (e _{marg. caud.} ) fort.Eine ähnliche areale Gradation wie im Gyrus parahippocampalis findet sich auch unter den vier Feldern des Gyrus ambiens. Das am höchsten organisierte Feld (ga _centr. ) liegt im caudalen und medialen Abschnitt und ist durch eine dreischichtige Lamina principalis interna und eine deutliche Lamina cellularis profunda ausgezeichnet. Im angrenzenden Feld ga _lat. ist Pri- stark reduziert. In ga _oral. findet sich nur eine einschichtige Lamina principalis interna. Der Grenzstreifen zum Mandelkernkomplex (e _{marg. oral.} ) besteht nur aus Teilen der äußeren Hauptschicht.Der breite Übergangsbereich von den rein allocorticalen Feldern der Regio entorhinalis bis zum Isocortex wird in vier Areae unterteilt, in denen allo- und isocorticale Schichten fugenartig ineinandergreifen. Die Stufungen ergeben sich dadurch, daß die einzelnen Zellamellen unterschiedlich weit vordringen. Eine modifizierte äußere Körnerschicht reicht bis in das Feld e _{trans. med.} ; zugleich wird Pre- in tiefer gelegene Rindenschichten verlagert. An der Grenze zu e _{trans. intermed.} endet Pre-. Die Spindelzellschicht beteiligt sich als ein weiteres isocorticales Element am Aufbau des intermediären Übergangsfeldes. Die seitlichen Kanten von Pre- und Pri- bilden die lineare Grenze zum lateralen Übergangsfeld, e _{trans. lat.} , dessen Struktur durch das Hinzutreten einer äußeren und inneren Pyramidenschicht bereits weitgehend dem Isocortex gleicht. Im Feld e _{trans. caud.} findet sich sowohl die Spindelzellschicht als auch Pre-. Es bildet damit eine Stufung zwischen dem medialen und intermediären Übergangsfeld, die jedoch nur im caudalen Abschnitt der Regio entorhinalis am Übergang zum Praesubiculum vorhanden ist.

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Pigmentarchitecture of the human cortex cerebriI. Regio entorhinalis

Summary By means of a newly developed method demonstrating neurolipofuscines the cellular layers constituting the regio entorhinalis are stained selectively. The differences between the individual cell types show up more clearly than in ordinary Nissl-preparations since by the new technique only one cytoplasmic component is stained. This limitation allows at the same time to use rather thick sections (up to 800 ), which — after clearing — are studied under the stereoscopic microscope. Thus indentations of neighbouring regions of the cortex and the edgelike formations of individual cortical layers can be demonstrated with certainty.The pigmentarchitecture of the allocortical layers differs clearly from that of the isocortex. The layers of the allocortex are not continuous with those of the isocortex. Within the regio entorhinalis the cortex can be divided into a lamina principalis externa (Pre) and a lamina principalis interna (Pri), which are separated by a narrow zone of fibers (lamina dissecans). The two main layers can be further subdivided (Pre-, Pre-, Pre-, Pri-, Pri-, Pri-).In the regio entorhinalis of man 16 areas can be distinguished by their pigmentarchitecture. 11 of these areas consist exclusively of allocortical layers, whereas the other areas which form the transitory part to the isocortex consist of various numbers of allo- and isocortical layers.In the region of the gyrus parahippocampalis 7 purely allocortical areas can be separated from each other. These areas are grouped in gradually decreasing levels of organisation round a highly differentiated center, which lies in oral and lateral parts of the regio entorhinalis. The characteristic feature of the central areas is a splitting of Pri- into three layers (Pri-, Pri-. Pri-). The area: e _{centr. lat.} contains all three sublayers of the lamina principalis externa, whereas in e _{centr. med.} Pre- is lacking. The neighbouring areas with uniform (not subdivided) Pri- can again be separated in areas with Pre- (e _{interpol. lat.} , e _caud. ) and a field without Pre- (e _{interpol. med.} ). In the rostral and medial parts Pri- and Pri- fuse forming an uniform cellular layer constituting the area: e _oral. . At the border of the gyrus ambiens near the sulcus rhinencephali inferior a narrow strip of cortex is to be found, in which the layers of the lamina principalis externa are only poorly developed. This limitrophic zone continues caudally into the border area to the praesubiculum (e _marg.caud. ).A similar areal gradation as in the gyrus parahippocampalis can be found in the four fields of the gyrus ambiens. The area with the highest organisation (ga _centr. ) is situated in the caudal and medial part of the gyrus ambiens and is characterised by a three layered lamina principalis interna and a clearly recognisable lamina cellularis profunda. In the neighbouring field ga _lat . Pri- is considerably reduced. In ga _oral. only an one layered lamina principalis interna is to be found. The border field to the amygdala (e _marg.oral. ) consists only of parts of the lamina principalis externa.The broad transitory region from the exclusively allocortical fields of the regio entorhinalis to the isocortex can be subdivided into four areas, in which allo- and isocortical layers meet in a zone of mutual indentations. The subdivision of the area is based on the different distances of penetration of the individual cellular layers. A modified lamina granularis externa extends into the field e _{trans. med.} ; at the same time Pre- is translocated into deeper cortical regions. At the border to e _{trans. intermed.} Pre- terminates. The lamina multiformis (VI) takes part as a further isocortical element in the construction of the area: e _{trans. intermed.} . The lateral edges of Pre- and Pri- form the linear border to the lateral transitory area (e _{trans. lat.} ), the structure of which resembles considerably that of the isocortex by additional appearance of a lamina pyramidalis externa and interna. In the area e _{trans. caud.} a lamina multiformis as well as the cellular layer Pre- is to be found, thus constituting a gradation between e _{trans. med.} and e _{trans. intermed.} , which, however, is present only in the caudal portions of the regio entorhinalis at the border to the praesubiculum.

Mit dankenswerter Unterstützung durch die Deutsche Forschungsgemeinschaft.     

Substructure of F1-ATPase (BF1 factor) from Micrococcus lysodeikticus

Summary Dimethyl suberimidate and dithiobis (succinimidyl propionate) have been used to explore the nearest neighbor relationship of the subunits (, , and by decreasing molecular weight) of F₁-ATPase or BF₁ factor of Micrococcus lysodeikticus. Cross-linking with the two diimido esters inhibited the ATPase activity but this inhibition never exceeded 50% of the initial value. The cross-linking pattern of this BF₁ factor, as revealed by sodium dodecyl sulfate gel electrophoresis, shows a relative low proportion of high molecular weight aggregates which move slowly than the heaviest subunit (). They are resolved as three components of molecular weights 200,000, 130,000 and 100,000 in 5% acrylamide gels, plus an additional component (mol. wt 80,000) identified in 10% acrylamide gels. The other aggregate bands represent cross-linking products of the smaller subunits ( and ) that may travel to the conventional position of the heavier subunits.The subunit composition of the aggregate bands has been determined through the reversion of dithiobis (succinimidyl propionate) cross-linking of the BF₁ factor by dithiothreitol and analysis in second dimension by gel electrophoresis. The results indicate that subunit can cross-link with itself and with each of the other subunits except . The subunit is also able to cross-link with itself and with the other subunits although to a minor extent than , and that ₂ aggregates are present. These results represent a specific pattern of cross-linking for this BF₁ factor as compared to other F₁ coupling factors. It suggests a certain asymmetry in the spatial organization of the major subunits of M. lysodeikticus F₁-ATPase where the subunit must play a central role. A subunit stoichiometry _{3 3 2 2} is proposed for whole F₁-ATPase which leads to a molecular weight 440,000 consistent with the 430,000 value estimated by sedimentation equilibrium at low speed. A tentative structural model of M. lysodeikticus BF₁ factor is derived from these data. The significance of the results in relation to the possible generalization of the molecular architecture of F₁ factors is discussed.     

Properties of theβ-glucosidase fromCellulomonas flavigena and fromEscherichia coli harboring the recombinant plasmid pJS3

Summary Plasmid-coded -glucosidase produced byEscherichia coli was characterized and compared to the enzyme produced byCellulomonas flavigena. Cell-free extracts, non-denaturing PAGE and 5-bromo-4-chloro-3-indolyl--d-glucopyranoside (X-glu) as substrate were used to compare both enzymes. The -glucosidase was assayed for cellobiose andp-nitrophenyl-glucopyranoside (PNPG). Cellobiose hydrolysis was performed at 50°C for the enzyme fromC. flavigena and at 37°C for that fromE. coli pJS3, both with an optimal pH of 6.5. For PNPG hydrolysis, the optimal conditions were pH 5.5 and 37°C for both cell extracts. Most of the -glucosidase activity was intracellular. When cultures ofC. flavigena were grown with cellobiose or carboxymethylcellulose (CMC) as inducers, the expression of -glucosidase was increased considerably.E. coli pJS3 produces a cellobiase which hydrolyzes cellobiose and PNPG. TheK _m values for cellobiose and PNPG indicated that the -glucosidase activity ofC. flavigena had a higher affinity for cellobiose as substrate, whereas the -glucosidase fromE. coli pJS3 showed higher affinity for PNPG.     

Immunofluorescence localization of α-amylase in the scutellum,germ aleurone and “normal” aleurone of germinated barley grains

Summary Using two step labeling with rhodamine-labeled secondary antibodies, -amylase (EC 3.2.1.1.) was detected in the scutellum, germ aleurone (monolayer partially encircling the scutellum) and normal aleurone (trilayer partially encircling the starchy endosperm; see Fulcher et al. 1972) in sections of Lowicryl-embedded barley (Hordeum vulgare L. cv. Himalaya) after imbibition of whole grains for 24, 48, and 72 h, but not after 2 h. Staining occurred over the protoplasts, cell walls or intercellular spaces of each tissue indicating that all three tissues had secreted as well as produced -amylase. The immunofluorescence in the scutellum was predominantly in the epithelium. Normal aleurone near the aleurone/ scutellum junction showed structural changes indicative of secretory activity by 24 h, and the pattern of cell erosion in the sub-aleurone and starchy endosperm at this and later stages supported this conclusion. The data show that normal aleurone is a major source of -amylase even at early stages of germination, but there is clear evidence also of production and secretion of some -amylase by both the scutellum and the germ aleurone, indicating that these tissues could also contribute to starch hydrolysis.Abbrevations GA₃ gibberellic acid - SDS sodium dodecyl sulphate - TBS 10 mM Tris, pH 7.4, containing 0.15 M NaCl - Tris 2-amino-2-(hydroxymethyl)-1, 3-propanediol     

Studies on lipase directed export of Escherichia coli beta-lactamase in Staphylococcus carnosus

Summary The lipase (lip) gene of Staphylococcus hyicus was used to study the expression of the Escherichia coli -lactamase (bla) gene in S. carnosus. The bla gene, devoid of its promotor and most of the signal sequence, was fused to the lip structural gene at various positions. A set of 11 secretion vectors (pLL1 to pLL11) was isolated and analysed. All secretion vectors caused -lactamase production and activity in S. carnosus. However, the amount of hybrid proteins secreted was influenced by the length of the NH₂-terminal lipase portion. An increased concentration, comparable to that of the native lipase, of secreted lipase/-lactamase hybrid proteins was only found when the lipase portion of the construct comprised more than 101 amino acids of the NH₂-terminal region of the lipase preprotein; the proposed lipase signal peptide is 36 amino acids long. If the hybrid proteins constructed contained 101 or less amino acids of the NH₂-terminal lipase preprotein, only low amounts of secreted hybrid proteins were detectable and a significant portion of the hybrid proteins and -lactamase activity was found in the cellular fraction. The results indicate that the lipase possesses adjacent to the signal peptide a peptide domain that is essential for the secretion of the lipase/-lactamase hybrid proteins.Abbreviations Cm chloramphenicol - bla gene beta lactamase coding gene of Escherichia coli - lip gene lipase-coding gene of Staphylococcus hyicus - PA polyacrylamide - PAGE PA gel electrophoresis - SDS sodium dodecyl sulphate - [] indicates plasmid-carrier state     

Lamivudine production via enantioselective deamination by thermostable Bacillus caldolyticus cytidine deaminase

To decrease the costs of producing the anti-HIV drug, lamivudine, an enzymatic conversion process was developed instead of the traditional chemical method. Thermostable cytidine deaminase was over-produced by cloning the cdd gene into E. coli JF611/pCJH53 from Bacillus caldolyticus. The purified cytidine deaminase was recovered from the lysate of the recombinant E. coli JF611/pCJH53 by removing heat-denatured proteins and eluting sequential chromatography. When the enzyme was used to deaminate (–)--l-(2R, 5S)- and (+)--d-(2S, 5R)-1, 3-oxathiolanyl-cytosine, about 68% of the (+)--d-(2S, 5R)-1, 3-oxathiolanyl-cytosine was deaminated into the corresponding (+)-thiauridine maximally.     

Changing glycine 21 for glutamic acid in the β-subunit of penicillin G acylase from Kluyvera citrophila prevents protein maturation

Summary Active penicillin acylase from Kluyvera citrophila strain ATCC 21 285 consists of two different -and -subunits derived from a single precursor by post-translational processing. Using the chemical mutagen hydroxylamine we have treated plasmid pYKD59 containing the active penicillin acylase gene (pga) from K. citrophila and have generated different point mutant penicillin acylase genes, one producing a muturation deficient precursor. This point mutation has changed the gylcine 310 residue of the precursor for a glutamic acid (residue number 21 of the mature -subunit). The introduction of a charged residue in this position did not prevent translocation of the precursor to the periplasm but the resultant molecule was not able to undergo subsequent post-translational modification to yield the active protein.     

Effect of deglycosylation on the properties of β-fructofuranosidaseP-1 fromAureobasidium sp. ATCC 20524

Summary Most of the carbohydrate moiety of -fructofuranosidaseP-1 fromAureobasidium sp. ATCC 20524 was removed by endo--N-acetylglucosaminidase F. A subunit of 94000 Da was observed in SDS-PAGE after deglycosylation. TheK _m value for sucrose was not changed by deglycosylation but the stability at pH 4–5 and 50°C was decreased. The deglycosylated enzyme was more sensitive to proteases such as pronase E and subtilisin than the native enzyme. It is considered that the carbohydrate moiety of -fructofuranosidaseP-1 contributes to the stability of the enzyme but is not essential in its catalytic function.     

Methanol and ethanol utilization in methylotrophic yeast Pichia pinus wild-type and mutant strains

In the wild-type strain of methylotrophic yeast Pichia pinus diauxic growth is observed during cultivation in medium containing a mixture of methanol and ethanol: firstly, slow phase of ethanol utilization is revealed and, secondly, a fast phase of methanol consumption is shown. Diauxic growth is observed also in ecr1 mutant, impaired in ethanol-induced catabolite repression of methylotrophic metabolism enzymes, but the order of utilization of the alcohols is inverted in this mutant. Such succession of alcohols utilization in both strains correlates well with the sequence of synthesis of microbody enzymes which catalyze key reactions of C₁- and C₂-metabolism. On the contrary, simultaneous utilization of methanol and ethanol from the mixture, as well as synchronous synthesis of both peroxisomal and glyoxisomal enzymes is observed in adh1 mutant which has reduced alcohol dehydrogenase activity. The strong differences between the wild-type strain and adh1 mutant were observed also in the kinetics of specific activity changes for C₁-metabolizing enzymes, localized in cytosol. In the wild-type strain during growth on methanol and ethanol mixture such changes correlate with the sequence of alcohol utilization. At the same time, in adh1 mutant the activities of formaldehyde dehydrogenase and formate dehydrogenase during the growth on the alcohols mixture are as high as during growth on methanol only, but the activity of dihydroxyacetone kinase is as low as under the growth on ethanol and is lower than on methanol.     

Characterization of recurrent somatic embryogenesis of alfalfa on auxin-free medium

Callus cultures from 300 genotypes of alfalfa (Medicago sativa L.) were initiated from leaf, petiole, and internode explants placed on Blaydes medium containing 10.74 M -naphthaleneacetic acid, 11.42 M indole-3-acetic acid, and 9.29 M kinetin. Five genotypes produced somatic embryos. Upon transfer of these embryos to growth regulator-free Murashige and Skoog medium with B₅ vitamins, new somatic embryos repeatedly formed directly on older somatic embryos without an intervening callus phase in a cycle lasting about 30 days. These cultures have been maintained for two years, during which time their embryogenic capacity has remained stable. New embryogenic cultures could be started repeatedly from these genotypes. The elimination of sugars from the medium could stop recurrent embryogenesis. Glucose, maltose, and fructose stimulated recurrent embryogenesis more effectively than sucrose. Sucrose was superior to lactose, while sorbitol and mannitol did not stimulate recurrent somatic embryogenesis. The absence of nicotinic acid in the medium, as long as sucrose was present, was lethal to embryos of three of the five tested genotypes. The ability of this system to propagate embryos exponentially offers potential for development of new gene transfer systems and application to artificial seed technology.Abbreviations NAA -naphthaleneacetic acid - RSE recurrent somatic embryogenesis     

Effects of α-galactosidase digestion on lectin staining in human pancreas

Summary Effects of -galactosidase (from green coffee beans) digestion on lectin staining were examined in formalin-fixed, paraffin-embedded human pancreatic tissues from individuals of blood-group B and AB. Digestion with the enzyme resulted in almost complete loss of Griffonia simplicifolia agglutinin I-B₄(GSAI-B₄) staining in the acinar cells with concomitant appearance of Ulex europaeus agglutinin-I(UEA-I) staining in the corresponding cells. In addition, reactivity with soybean agglutinin(SBA) was also imparted by the enzyme digestion in GSAI-B₄ positive acinar cells. -Galactosidase digestion following -galactosidase digestion neither reduced the reactivity with SBA nor induced the reactivity with Griffonia simplicifolia agglutinin-II(GSA-II) in GSAI-B₄ positive cells, while in UEA-I positive cells, both reduction of SBA reactivity and appearance of GSA-II reactivity occurred after simple -galactosidase digestion as well as sequential digestion with - and -galactosidase. However, when -l-fucosidase digestion procedure was inserted between - and -galactosidase digestion, UEA-I staining imparted by -galactosidase digestion was markedly decreased in intensity and GSA-II reactivity was appeared in GSAI-B₄ positive acinar cells. Furthermore, after sequential digestion with -galactosidase and fucosidase, reactivity with peanut agglutinin(PNA) was revealed in GSAI-B₄ positive acinar cells as well as UEA-I positive cells in secretors. In non-secretors, strong PNA staining was usually observed in the acinar cells throughout the glands without enzyme digestion. These results confirmed that the -galactosidase induced GSA-II reactivity and the fucosidase induced PNA reactivity are due to precursors of different kinds of blood-group determinants and suggest that at least two kinds of B antigen determinants, i.e. Gal(1-3)[Fuc(1-2)]Gal(1-3,4)GlcNac and Gal(1-3)-[Fuc(1-2)]Gal(1-3)GalNAc are produced in GSAI-B₄ positive acinar cells. The synthesis of the latter type of B antigen is assumed to be controlled under the secretory gene in human pancreas.Abbreviation GalNAc N-acetyl-d-galactosamine - Gal d-galactose - GlcNAc N-acetyl-d-glucosamine - Fuc l-fucose - NeuNAc N-acetylneuraminic acid (sialic acid)