Different glycan structures in prostate-specific antigen from prostate cancer sera in relation to seminal plasma PSA

Tabarés, Glòria; Radcliffe, Catherine M.; Barrabés, Sílvia; Ramírez, Manel; Aleixandre, Rosa Núria; Hoesel, Wolfgang; Dwek, Raymond A.; Rudd, Pauline M.; Peracaula, Rosa; Llorens, Rafael de

doi:10.1093/glycob/cwj042

Cited by 151 publications

(174 citation statements)

References 42 publications

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“…Here, we quantify endogenous PSA isoforms present in 3 μL of minimally processed lysate from LAPC-4 cells derived from a lymph node of a human prostate cancer patient. The probed LAPC-4 lysate presents a distinctive four peak pattern in the pI 6.9-7.9 range that is similar to slab-gel assays of PSA purified from LAPC-4 cell culture medium (8,30). As a negative control, lysate from a PSA negative cell line (DU145) was assayed and shows no detectable PSA isoform readout, as expected.…”

Section: Resultssupporting

confidence: 66%

“…The two PSA+ samples each show three major PSA isoforms falling within the pI 6.4-7.5 range, in good agreement with comparatively laborious slab-gel IEF studies (6,8). Patient-specific differences in PSA isoform representation and pI are clearly apparent, recapitulating the potential utility of isoform ratio measurements in clinical diagnostics and personalized medicine (6,7).…”

Section: Microfluidic Lavagel Analysis Of Psa Isoforms In Metastatic supporting

confidence: 65%

“…Proteomic studies suggest a promising link between prostate cancer incidence and differential isoform expression in healthy and cancer patient sera (6,8,9). Although promising, rigorous validation studies are needed to translate the potential of protein isoforms to the clinic.…”

mentioning

confidence: 99%

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Microfluidic integration for automated targeted proteomic assays

Hughes

Lin

Peehl

et al. 2012

Proc. Natl. Acad. Sci. U.S.A.

103

167

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A dearth of protein isoform-based clinical diagnostics currently hinders advances in personalized medicine. A well-organized protein biomarker validation process that includes facile measurement of protein isoforms would accelerate development of effective protein-based diagnostics. Toward scalable protein isoform analysis, we introduce a microfluidic "single-channel, multistage" immunoblotting strategy. The multistep assay performs all immunoblotting steps: separation, immobilization of resolved proteins, antibody probing of immobilized proteins, and all interim wash steps. Programmable, low-dispersion electrophoretic transport obviates the need for pumps and valves. A three-dimensional bulk photoreactive hydrogel eliminates manual blotting. In addition to simplified operation and interfacing, directed electrophoretic transport through our 3D nanoporous reactive hydrogel yields superior performance over the state-of-the-art in enhanced capture efficiency (on par with membrane electroblotting) and sparing consumption of reagents (ca. 1 ng antibody), as supported by empirical and by scaling analyses. We apply our fully integrated microfluidic assay to protein measurements of endogenous prostate specific antigen isoforms in (i) minimally processed human prostate cancer cell lysate (1.1 pg limit of detection) and (ii) crude sera from metastatic prostate cancer patients. The single-instrument functionality establishes a scalable microfluidic framework for high-throughput targeted proteomics, as is relevant to personalized medicine through robust protein biomarker verification, systematic characterization of new antibody probes for functional proteomics, and, more broadly, to characterization of human biospecimen repositories.isoelectric focusing | nanoporous reactive polymers | lab-on-a-chip | Western blotting | antibody selection

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Section: Resultssupporting

confidence: 66%

Section: Microfluidic Lavagel Analysis Of Psa Isoforms In Metastatic supporting

confidence: 65%

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Microfluidic integration for automated targeted proteomic assays

Hughes

Lin

Peehl

et al. 2012

Proc. Natl. Acad. Sci. U.S.A.

103

167

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“…There is increasing evidence that the PSA glycosylation is altered in prostate cancer serum in comparison to normal PSA [24,25]. Fig.…”

Section: Prostate-specific Antigen (Psa)mentioning

confidence: 99%

A lectin array-based methodology for the analysis of protein glycosylation

Rosenfeld¹,

Bangio²,

Gerwig³

et al. 2007

Journal of Biochemical and Biophysical Methods

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Glycosylation is the most versatile and one of the most abundant protein modifications. It has a structural role as well as diverse functional roles in many specific biological functions, including cancer development, viral and bacterial infections, and autoimmunity. The diverse roles of glycosylation in biological processes are rapidly growing areas of research, however, Glycobiology research is limited by the lack of a technology for rapid analysis of glycan composition of glycoproteins. Currently used methods for glycoanalysis are complex, typically requiring high levels of expertise and days to provide answers, and are not readily available to all researcher.We have developed a lectin array-based method, Qproteome™ GlycoArray kits, for rapid analysis of glycosylation profiles of glycoproteins. Glycoanalysis is performed on intact glycoproteins, requiring only 4-6 h for most analysis types. The method, demonstrated in this manuscript by several examples, is based on binding of an intact glycoprotein to the arrayed lectins, resulting in a characteristic fingerprint that is highly sensitive to changes in the protein's glycan composition. The large number of lectins, each with its specific recognition pattern, ensures high sensitivity to changes in the glycosylation pattern. A set of proprietary algorithms automatically interpret the fingerprint signals to provide a comprehensive glycan profile output.

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“…Also, the glycosylation of prostate cancer KLK3 was reduced in benign prostate hyperplasia (BPH) and exhibited a different composition (Basu et al, 2003;Ohyama et al, 2004) KLK3 from prostate tumor cell lines shows an altered sugar composition, with a significant lack of sialic acid in the N-glycan tree (Peracaula et al, 2003). Seemingly, differences exist in fucosylation and sialylation of KLK3 from prostate cancer patients, although they do not appear to be sufficient for reliable prognosis of the disease (Tabares et al, 2006(Tabares et al, , 2007. Nevertheless, these differences have the potential to discriminate between benign and malignant prostate disease, e.g., by monitoring the complex of KLK3 with anti-chymotrypsin, by using fucosylation analysis, mass spectrometry or lectin microarrays and immunosorbent assays (Tajiri et al, 2008;Dwek et al, 2010;Sarrats et al, 2010;Yan Li et al, 2011).…”

Section: The Prostatic Klks 2 Andmentioning

confidence: 99%

Sweetened kallikrein-related peptidases (KLKs): glycan trees as potential regulators of activation and activity

Guo

Skala

Magdolen

et al. 2014

Biological Chemistry

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Most kallikrein-related peptidases (KLKs) are N-glycosylated with N-acetylglucosamine 2 -mannose 9 units at Asn-Xaa-Ser/Thr sequons during protein synthesis and translocation into the endoplasmic reticulum. These N-glycans are modified in the Golgi machinery, where additional O-glycosylation at Ser and Thr takes place, before exocytotic release of the KLKs into the extracellular space. Sequons are present in all 15 members of the KLKs and comparative studies for KLKs from natural and recombinant sources elucidated some aspects of glycosylation. Although glycosylation of mammalian KLKs 1, 3, 4, 6, and 8 has been analyzed in great detail, e.g., by crystal structures, the respective function remains largely unclear. In some cases, altered enzymatic activity was observed for KLKs upon glycosylation. Remarkably, for KLK3/PSA, changes in the glycosylation pattern were observed in samples of benign prostatic hyperplasia and prostate cancer with respect to healthy individuals. Potential functions of KLK glycosylation in structural stabilization, protection against degradation, and activity modulation of substrate specificity can be deduced from a comparison with other glycosylated proteins and their regulation. According to the new concept of protein sectors, glycosylation distant from the active site might significantly influence the activity of proteases. Novel pharmacological approaches can exploit engineered glycans in the therapeutical context.

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Different glycan structures in prostate-specific antigen from prostate cancer sera in relation to seminal plasma PSA

Cited by 151 publications

References 42 publications

Microfluidic integration for automated targeted proteomic assays

Microfluidic integration for automated targeted proteomic assays

A lectin array-based methodology for the analysis of protein glycosylation

Sweetened kallikrein-related peptidases (KLKs): glycan trees as potential regulators of activation and activity

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