The activation pathway of procarboxypeptidase B from porcine pancreas: Participation of the active enzyme in the proteolytic processing

Villegas, Sandra; Vendrell, Josep; Avilés, Xavier

doi:10.1002/pro.5560040914

Cited by 28 publications

(22 citation statements)

References 29 publications

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“…The recombinant pro-CPB was fully activated when incubated at 0°C and at 400/1 pro-CPB/trypsin (w/w) ratio. The maturation course for recombinant pro-CPB is identical to that previously reported for the natural form isolated from porcine pancreas (16). A scheme of the proteolytic maturation process is presented in Fig.…”

Section: Figsupporting

confidence: 72%

“…The supernatant was loaded onto a hydrophobic interaction butyl column and eluted with a decreasing gradient of ammonium sulfate. The zymogen-containing fractions were selected for their activity against BGA after tryptic activation and re-purified by fast protein liquid chromatography on an anion exchange column (TSK-DEAE) as reported previously (16). The correct processing of the different recombinant proteins was confirmed by both automated Edman degradation analysis of its N-terminal sequence and mass spectrometry.…”

Section: Methodsmentioning

confidence: 99%

“…3). Previous studies have shown that Arg-93 may also act as a primary tryptic target when carboxypeptidase inhibitors are added to the activation mixture (16).…”

Section: Figmentioning

confidence: 99%

“…At the top of the figure, the sequence around the primary and secondary processing sites is presented to serve as a guide. Modified from Villegas et al (16).…”

Section: Fig 2 Schematic View Of the Sequence Of Cleavages Observedmentioning

confidence: 99%

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Mapping the Pro-region of Carboxypeptidase B by Protein Engineering

Ventura¹,

Villegas²,

Sterner³

et al. 1999

Journal of Biological Chemistry

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The proteolytic processing of pancreatic procarboxypeptidase B to a mature and functional enzyme is much faster than that of procarboxypeptidase A1. This different behavior has been proposed to depend on specific conformational features at the region that connects the globular domain of the pro-segment to the enzyme and at the contacting surfaces on both moieties. A cDNA coding for porcine procarboxypeptidase B was cloned, sequenced, and expressed at high yield (250 mg/liter) in the methylotrophic yeast Pichia pastoris. To test the previous hypothesis, different mutants of the pro-segment at the putative tryptic targets in its connecting region and at some of the residues contacting the active enzyme were obtained. Moreover, the complete connecting region was replaced by the homologous sequence in procarboxypeptidase A1. The detailed study of the tryptic processing of the mutants shows that limited proteolysis of procarboxypeptidase B is a very specific process, as Arg-95 is the only residue accessible to tryptic attack in the proenzyme. A fast destabilization of the connecting region after the first tryptic cut allows subsequent proteolytic processing and the expression of carboxypeptidase B activity. Although all pancreatic procarboxypeptidases have a preformed active site, only the A forms show intrinsic activity. Mutational substitution of Asp-41 in the globular activation domain, located at the interface with the enzyme moiety, as well as removal of the adjacent 3 10 helix allow the appearance of residual activity in the mutated procarboxypeptidase B, indicating that the interaction of both structural elements with the enzyme moiety prevents the binding of substrates and promotes enzyme inhibition. In addition, the poor heterologous expression of such mutants indicates that the mutated region is important for the folding of the whole proenzyme.

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Section: Figsupporting

confidence: 72%

Section: Methodsmentioning

confidence: 99%

“…3). Previous studies have shown that Arg-93 may also act as a primary tryptic target when carboxypeptidase inhibitors are added to the activation mixture (16).…”

Section: Figmentioning

confidence: 99%

“…At the top of the figure, the sequence around the primary and secondary processing sites is presented to serve as a guide. Modified from Villegas et al (16).…”

Section: Fig 2 Schematic View Of the Sequence Of Cleavages Observedmentioning

confidence: 99%

See 2 more Smart Citations

Mapping the Pro-region of Carboxypeptidase B by Protein Engineering

Ventura¹,

Villegas²,

Sterner³

et al. 1999

Journal of Biological Chemistry

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“…Folding studies performed in ADA2h showed an extremely fast two-state kinetics [6], suggesting that ADs could assist in the proenzyme folding. Supporting this hypothesis, recombinant expressions of various forms of CPs in the methylotrophic yeast Pichia pastoris have been proved unsuccessful, whereas the proenzyme forms can be produced at high yields.…”

Section: Introductionmentioning

confidence: 98%

Prediction of a new class of RNA recognition motif

Cerdà-Costa¹,

Bonet²,

Fernández³

et al. 2010

J Mol Model

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The observation that activation domains (AD) of procarboxypeptidases are rather long, compared to pro-regions of other zymogens, points out the possibility that they could play additional roles apart from precluding enzymatic activity within the proenzyme and helping in its folding process. In the present work, we have compared the overall pro-domain tertiary structure with several proteins belonging to the same fold in SCOP by using structure and sequence comparisons. The best score has been obtained between the activation domain of the human procarboxypeptidase A4 (ADA4h) and the human U1A protein from the U1 snRNP.Structural alignment has revealed the existence of RNP1-and RNP2-related sequences in ADA4h. After modeling ADA4h on U1A, the new structure was used to extract a new sequence pattern characteristic for important residues at key positions. The new sequence pattern allowed scanning protein sequences to predict the RNA-binding function for 32 sequences undetected by PFAM. Unspecific RNA EMSA experimentally supported the prediction that ADA4h binds an RNA motif similar to the U1A binding-motif of stem-loop II of U1 small nuclear RNA. The experiments carried out with ADA4h in the present work Manuscript Click here to download Manuscript: JMMO1391R2_final.doc 2 suggest the sharing of a common ancestor with other RRMs. However, the fact that key residues preventing activity within the proenzyme are also key residues for RNA binding might induce the activation domains of procarboxypeptidases to evolve from the canonical RNP1 and 2 sequences.

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Probing of C‐terminal lysine variation in a recombinant monoclonal antibody production using Chinese hamster ovary cells with chemically defined media

Luo

Zhang

Ren

et al. 2012

Biotech & Bioengineering

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C-terminal lysine (C-K) variants are commonly observed in therapeutic monoclonal antibodies and recombinant proteins. Heterogeneity of C-K residues is believed to result from varying degree of proteolysis by endogenous carboxypeptidase(s) during cell culture production. The achievement of batch-to-batch culture performance and product quality reproducibility is a key cell culture development criterion. Understanding the operational parameters affecting C-K levels provides valuable insight into the cell culture process. A CHO cell line X expressing a recombinant antibody was selected as the model cell line due to the exhibited sensitivity of its C-K level to the process conditions. A weak cation exchange chromatography (WCX) method with or without carboxypeptidase B (CpB) treatment was developed to monitor the C-K level for in-process samples. The effects of operating conditions (i.e., temperature and culture duration) and media trace elements (copper and zinc) on C-K variants were studied. The dominant effect on C-K level was identified as the trace elements concentration. Specifically, increased C-K levels were observed with increase of copper concentration and decrease of zinc concentration in chemically defined medium. Further, a hypothesis for C-K processing with intracellular and extracellular carboxypeptidase activity was proposed, based on preliminary intracellular carboxypeptidase Western blot results and the extracellular HCCF holding study.

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The activation pathway of procarboxypeptidase B from porcine pancreas: Participation of the active enzyme in the proteolytic processing

Cited by 28 publications

References 29 publications

Mapping the Pro-region of Carboxypeptidase B by Protein Engineering

Mapping the Pro-region of Carboxypeptidase B by Protein Engineering

Prediction of a new class of RNA recognition motif

Probing of C‐terminal lysine variation in a recombinant monoclonal antibody production using Chinese hamster ovary cells with chemically defined media

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