Biosynthesis of intestinal microvillar proteins. Processing of aminopeptidase N by microsomal membranes

The biosynthesis of small-intestinal aminopeptidase N (EC 3.4.11.2) was studied in a cell-free translation system derived from rabbit reticulocytes. When dog pancreatic microsomal fractions were present during translation, most of the aminopeptidase N synthesized was found in a membrane-bound rather than a soluble form, indicating that synthesis of the enzyme takes place on ribosomes attached to the rough endoplasmic reticulum. The microsomal fractions process the Mr-115 000 polypeptide, which is the primary translation product of aminopeptidase N, to a polypeptide of Mr 140 000. This was found to be sensitive to the action of endo-beta-N-acetylglucosaminidase H (EC 3.2.1.96), showing that aminopeptidase N undergoes transmembrane glycosylation during synthesis. The position of the signal sequence in aminopeptidase N was determined by a synchronized translation experiment. It was found that microsomal fractions should be added before about 25% of the polypeptide was synthesized to ensure processing to the high-mannose glycosylated form. This suggests that the signal sequence is situated in the N-terminal part of the aminopeptidase N. The size of the cell-free translation product in the absence of microsomal fractions was found to be similar to that on one of the forms of the enzyme obtained from tunicamycin-treated organ-cultured intestinal explants.

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The microsomal epoxide hydrolase has a single membrane signal anchor sequence which is dispensable for the catalytic activity of this protein

Biochemical Journal ◽

10.1042/bj3030967 ◽

1994 ◽

Vol 303 (3) ◽

pp. 967-972 ◽

Cited By ~ 29

Author(s):

T Friedberg ◽

B Löllmann ◽

R Becker ◽

R Holler ◽

F Oesch

Keyword(s):

Catalytic Activity ◽

Amino Acid ◽

Fusion Protein ◽

Epoxide Hydrolase ◽

Signal Sequence ◽

Translation System ◽

Amino Acid Residues ◽

Membrane Anchor ◽

Free Translation ◽

A Cell

The microsomal epoxide hydrolase (mEH) catalyses the hydrolysis of reactive epoxides which are formed by the action of cytochromes P-450 from xenobiotics. In addition it has been suggested that mEH might mediate the transport of bile acids. For the mEH it has been shown that it is co-translationally inserted into the endoplasmic reticulum. Here we demonstrate that the N-terminal 20 amino acid residues of this protein serve as its single membrane anchor signal sequence and that the function of this sequence can also be supplied by a cytochrome P-450 (CYP2B1) anchor signal sequence. The evidence supporting this conclusion is as follows: (i) the rat mEH and a CYP2B1-mEH fusion protein, in which the CYP2B1 membrane anchor signal sequence replaced the N-terminal 20 amino acid residues of mEH, was co-translationally inserted into dog pancreas microsomes in a cell-free translation system, whereas a truncated epoxide hydrolase with a deletion of the 20 N-terminal amino acid residues was not co-translationally inserted. (ii) The mEH and the CYP2B1-mEH fusion protein, but not the truncated epoxide hydrolase, were anchored in microsomes in a cell-free translation system and in membrane fractions derived from fibroblasts which expressed these proteins heterologously. These fibroblasts were also used to evaluate the significance of the mEH membrane anchor for the catalytic activity of mEH. The mEH, the truncated mEH and the CYP-EH fusion protein were found to be enzymically active. This result shows that the membrane anchor signal sequence of mEH is dispensable for the catalytic activity of this protein. However, truncated mEH was only expressed at low levels, which might indicate that this protein is unstable.

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Induction of cytochrome P-450 by pregnenolone-16 alpha-carbonitrile in primary monolayer cultures of adult rat hepatocytes and in a cell-free translation system.

Journal of Biological Chemistry ◽

10.1016/s0021-9258(19)69128-3 ◽

1981 ◽

Vol 256 (12) ◽

pp. 6060-6068

Author(s):

N.A. Elshourbagy ◽

J.L. Barwick ◽

P.S. Guzelian

Keyword(s):

Rat Hepatocytes ◽

Translation System ◽

Adult Rat ◽

Monolayer Cultures ◽

Adult Rat Hepatocytes ◽

Free Translation ◽

A Cell ◽

Primary Monolayer ◽

Cytochrome P 450 ◽

Primary Monolayer Cultures

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The 3' untranslated region of satellite tobacco necrosis virus RNA stimulates translation in vitro.

Molecular and Cellular Biology ◽

10.1128/mcb.13.6.3340 ◽

1993 ◽

Vol 13 (6) ◽

pp. 3340-3349 ◽

Cited By ~ 68

Author(s):

X Danthinne ◽

J Seurinck ◽

F Meulewaeter ◽

M Van Montagu ◽

M Cornelissen

Keyword(s):

Tobacco Necrosis Virus ◽

Translation System ◽

Coding Region ◽

Necrosis Virus ◽

Untranslated Sequence ◽

Virus Rna ◽

Free Translation ◽

Order Of Magnitude ◽

A Cell

The RNA of satellite tobacco necrosis virus (STNV) is a monocistronic messenger that lacks both a 5' cap structure and a 3' poly(A) tail. We show that in a cell-free translation system derived from wheat germ, STNV RNA lacking the 600-nucleotide trailer is translated an order of magnitude less efficiently than full-size RNA. Deletion analyses positioned the translational enhancer domain (TED) within a conserved hairpin structure immediately downstream from the coat protein cistron. TED enhances translation when fused to a heterologous mRNA, but the level of enhancement depends on the nature of the 5' untranslated sequence and is maximal in combination with the STNV leader. The STNV leader and TED have two regions of complementarity. One of the complementary regions in TED resembles picornavirus box A, which is involved in cap-independent translation but which is located upstream of the coding region.

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Easy and Rapid Binding Assay for Functional Analysis of Disulfide-Containing Peptides by a Pull-Down Method Using a Puromycin-Linker and a Cell-Free Translation System

Biology ◽

10.3390/biology4010161 ◽

2015 ◽

Vol 4 (1) ◽

pp. 161-172 ◽

Cited By ~ 2

Author(s):

Yutaro Tanemura ◽

Yuki Mochizuki ◽

Shigefumi Kumachi ◽

Naoto Nemoto

Keyword(s):

Functional Analysis ◽

Binding Assay ◽

Translation System ◽

Free Translation ◽

A Cell ◽

Rapid Binding

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A murine fer testis-specific transcript (ferT) encodes a truncated Fer protein.

Molecular and Cellular Biology ◽

10.1128/mcb.10.1.146 ◽

1990 ◽

Vol 10 (1) ◽

pp. 146-153 ◽

Cited By ~ 56

Author(s):

K Fischman ◽

J C Edman ◽

G M Shackleford ◽

J A Turner ◽

W J Rutter ◽

...

Keyword(s):

Tyrosine Kinase ◽

Translation System ◽

Appearance Time ◽

Acid Protein ◽

Mouse Tissues ◽

Free Translation ◽

Alternatively Spliced ◽

A Cell ◽

Testis Cdna ◽

Carboxy Terminal

A cDNA for a potential tyrosine kinase-encoding mRNA was isolated from a mouse testis cDNA library. In a survey of eight mouse tissues, a transcript of 2.4 kilobases restricted to testis tissue was found. The mRNA encodes a 453-amino-acid protein of 51,383 daltons, the smallest tyrosine kinase protein ever described. RNA synthesized from the cDNA template directs the synthesis of a 51,000-Mr protein in a cell-free translation system. The carboxy-terminal 409 amino acids are 98 and 90% identical to the carboxy halves of the rat and human Fer proteins, respectively. This suggests that the cDNA represents an alternatively spliced testis-specific fer mRNA and is therefore termed by us ferT. On the basis of the appearance time of the fer mRNA in the testis of maturing neonatal mice, we speculate on the role played by this protein in the development of this organ.

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Chemical aminoacylation of tRNAs with fluorinated amino acids for in vitro protein mutagenesis

Beilstein Journal of Organic Chemistry ◽

10.3762/bjoc.6.40 ◽

2010 ◽

Vol 6 ◽

Cited By ~ 8

Author(s):

Shijie Ye ◽

Allison Ann Berger ◽

Dominique Petzold ◽

Oliver Reimann ◽

Benjamin Matt ◽

...

Keyword(s):

Amino Acids ◽

Translation System ◽

Biologically Relevant ◽

Fluorinated Amino Acids ◽

Free Translation ◽

Trna Species ◽

A Cell ◽

Protein Environment ◽

Vitro Protein

This article describes the chemical aminoacylation of the yeast phenylalanine suppressor tRNA with a series of amino acids bearing fluorinated side chains via the hybrid dinucleotide pdCpA and ligation to the corresponding truncated tRNA species. Aminoacyl-tRNAs can be used to synthesize biologically relevant proteins which contain fluorinated amino acids at specific sites by means of a cell-free translation system. Such engineered proteins are expected to contribute to our understanding of discrete fluorines’ interaction with canonical amino acids in a native protein environment and to enable the design of fluorinated proteins with arbitrary desired properties.

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Ribosome binding to the endoplasmic reticulum: a 180-kD protein identified by crosslinking to membrane-bound ribosomes is not required for ribosome binding activity.

The Journal of Cell Biology ◽

10.1083/jcb.114.4.639 ◽

1991 ◽

Vol 114 (4) ◽

pp. 639-649 ◽

Cited By ~ 30

Author(s):

P G Collins ◽

R Gilmore

Keyword(s):

Signal Sequence ◽

Signal Recognition Particle ◽

Membrane Vesicles ◽

Immunoblot Analysis ◽

Binding Activity ◽

Size Exclusion ◽

Ribosome Binding ◽

Specific Subset ◽

Microsomal Membranes ◽

Membrane Bound

We have used the membrane-impermeable, thiol-cleavable, crosslinker 3,3'-dithio bis (sulfosuccinimidylpropionate) to identify proteins that are in the vicinity of membrane-bound ribosomes of the RER. A specific subset of RER proteins was reproducibly crosslinked to the ribosome. Immunoblot analysis of the crosslinked products with antibodies raised against signal recognition particle receptor, ribophorin I, and the 35-kD subunit of the signal sequence receptor demonstrated that these translocation components had been crosslinked to the ribosome, but each to a different extent. The most prominent polypeptide among the crosslinked products was a 180-kD protein that has recently been proposed to be a ribosome receptor (Savitz, A.J., and D.I. Meyer, 1990. Nature (Lond.). 346: 540-544). RER membrane proteins were reconstituted into liposomes and assayed with radiolabeled ribosomes to determine whether ribosome binding activity could be ascribed to the 180-kD protein. Differential detergent extraction was used to prepare soluble extracts of microsomal membrane vesicles that either contained or lacked the 180-kD protein. Liposomes reconstituted from both extracts bound ribosomes with essentially identical affinity. Additional fractionation experiments demonstrated that the bulk of the ribosome binding activity present in detergent extracts of microsomal membranes could be readily resolved from the 180-kD protein by size exclusion chromatography. Taken together, we conclude that the 180-kD protein is in the vicinity of membrane bound ribosomes, yet does not correspond to the ribosome receptor.

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Biosynthesis of intestinal microvillar proteins. Pulse-chase labelling studies on maltase-glucoamylase, aminopeptidase A and dipeptidyl peptidase IV

Biochemical Journal ◽

10.1042/bj2100389 ◽

1983 ◽

Vol 210 (2) ◽

pp. 389-393 ◽

Cited By ~ 23

Author(s):

E M Danielsen ◽

H Sjöström ◽

O Norén

Keyword(s):

Organ Culture ◽

Membrane Fraction ◽

Bound State ◽

Dipeptidyl Peptidase ◽

Dipeptidyl Peptidase Iv ◽

Soluble Form ◽

Membrane Bound ◽

Aminopeptidase A ◽

High Mannose ◽

Small Intestinal

The biogenesis of three intestinal microvillar enzymes, maltase-glucoamylase (EC 3.2.1.20), aminopeptidase A (aspartate aminopeptidase, EC 3.4.11.7) and dipeptidyl peptidase IV (EC 3.4.14.5), was studied by pulse-chase labelling of pig small-intestinal explants kept in organ culture. The earliest detectable forms of the enzymes were polypeptides of Mr 225000, 140000 and 115000 respectively. These were found to represent the enzymes in a ‘high-mannose’ state of glycosylation, as judged by their susceptibility to treatment with endo-beta-N-acetylglucosaminidase H (EC 3.2.1.96). After about 40-60 min of chase, maltase-glucoamylase, aminopeptidase A and dipeptidyl peptidase IV were further modified to yield the mature polypeptides of Mr 245000, 170000 and 137000 respectively, which were expressed at the microvillar membrane after 60-90 min of chase. The fact that the enzymes before reaching the microvillar membrane were found in a Ca2+-precipitated membrane fraction (intracellular and basolateral membranes), but not in soluble form, indicates that during biogenesis maltase-glucoamylase, aminopeptidase A and dipeptidyl peptidase IV are transported and assembled in a membrane-bound state.

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Studies of the Biosynthesis of Renin with a Cell-Free Translation System

Clinical Science ◽

10.1042/cs061241s ◽

1981 ◽

Vol 61 (s7) ◽

pp. 241s-243s ◽

Cited By ~ 3

Author(s):

V. J. Dzau ◽

A. Ouellette ◽

R. Pratt

Keyword(s):

Molecular Weight ◽

Polyacrylamide Gel Electrophoresis ◽

Submaxillary Gland ◽

Translation System ◽

Mouse Submaxillary Gland ◽

Free Translation ◽

Renin Mrna ◽

A Cell ◽

Deficient Mice ◽

Identical Fashion

1. Poly(A)+ mRNA from mouse submaxillary gland encodes a polypeptide of molecular weight 48 000 (48K polypeptide) which is abundant in the male. 2. This polypeptide is selectively absent in the translation products of mRNA from a strain of genetically renin-deficient mice C57 BL/10J. 3. The 48K polypeptide binds and co-elutes in identical fashion with pure authentic renin on pepstatin affinity chromatography. 4. Immunoprecipitation of translation products of male glandular mRNA with renin-specific antibody yielded this 48K band upon analysis by SDS/polyacrylamide gel electrophoresis and fluorography. Pure renin of molecular weight 37 000 blocked the binding of this polypeptide to antirenin antibody. 5. Mouse submaxillary gland synthesizes a renin precursor. The renin mRNA is androgenically regulated.

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Reconstitution of functional mRNA-protein complexes in a rabbit reticulocyte cell-free translation system.

Molecular and Cellular Biology ◽

10.1128/mcb.5.2.342 ◽

1985 ◽

Vol 5 (2) ◽

pp. 342-351 ◽

Cited By ~ 28

Author(s):

J R Greenberg ◽

E Carroll

Keyword(s):

Mammalian Cells ◽

Uv Light ◽

Protein Complexes ◽

Micrococcal Nuclease ◽

Translation System ◽

Cytoplasmic Process ◽

Free Translation ◽

Associated Proteins ◽

A Cell ◽

And Function

A variety of evidence suggests that the cytoplasmic mRNA-associated proteins of eucaryotic cells are derived from the cytoplasm and function there, most likely in protein synthesis or some related process. Furthermore, the evidence suggests that protein-free mRNA added to a cell-free translation system should become associated with a set of proteins similar to those associated with mRNA in native polyribosomes. To test this hypothesis, we added deproteinized rabbit reticulocyte mRNA to a homologous cell-free translation system made dependent on exogenous mRNA by treatment with micrococcal nuclease. The resulting reconstituted complexes were irradiated with UV light to cross-link the proteins to mRNA, and the proteins were analyzed by gel electrophoresis. The proteins associated with polyribosomal mRNA in the reconstituted complexes were indistinguishable from those associated with polyribosomal mRNA in intact reticulocytes. Furthermore, reticulocyte mRNA-associated proteins were very similar to those of cultured mammalian cells. The composition of the complexes varied with the translational state of the mRNA; that is, certain proteins present in polyribosomal mRNA-protein complexes were absent or reduced in amount in 40S to 80S complexes and in complexes formed in the absence of translation. However, other proteins, including a 78-kilodalton protein associated with polyadenylate, were present irrespective of translational state, or else they were preferentially associated with untranslated mRNA. These findings are in agreement with previous data suggesting that proteins associated with cytoplasmic mRNA are derived from the cytoplasm and that they function in translation or some other cytoplasmic process, rather than transcription, RNA processing, or transport from the nucleus to the cytoplasm.

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