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17 results on '"Görnemann, Janina"'

1. When monoclonal antibodies are not monospecific: Hybridomas frequently express additional functional variable regions

Author

Bradbury, Andrew RM, Trinklein, Nathan D, Thie, Holger, Wilkinson, Ian C, Tandon, Atul K, Anderson, Stephen, Bladen, Catherine L, Jones, Brittany, Aldred, Shelley Force, Bestagno, Marco, Burrone, Oscar, Maynard, Jennifer, Ferrara, Fortunato, Trimmer, James S, Görnemann, Janina, Glanville, Jacob, Wolf, Philipp, Frenzel, Andre, Wong, Julin, Koh, Xin Yu, Eng, Hui-Yan, Lane, David, Lefranc, Marie-Paule, Clark, Mike, and Dübel, Stefan

Subjects
Immunization, Genetics, Vaccine Related, Biotechnology, Animals, Antibodies, Monoclonal, Antibody Specificity, Genes, Immunoglobulin Heavy Chain, Genes, Immunoglobulin Light Chain, Humans, Hybridomas, hybridoma, monoclonal antibodies, specificity, paratope, recombinant antibodies, Immunology, Pharmacology and Pharmaceutical Sciences, Public Health and Health Services
Abstract

Monoclonal antibodies are commonly assumed to be monospecific, but anecdotal studies have reported genetic diversity in antibody heavy chain and light chain genes found within individual hybridomas. As the prevalence of such diversity has never been explored, we analyzed 185 random hybridomas, in a large multicenter dataset. The hybridomas analyzed were not biased towards those with cloning difficulties or known to have additional chains. Of the hybridomas we evaluated, 126 (68.1%) contained no additional productive chains, while the remaining 59 (31.9%) contained one or more additional productive heavy or light chains. The expression of additional chains degraded properties of the antibodies, including specificity, binding signal and/or signal-to-noise ratio, as determined by enzyme-linked immunosorbent assay and immunohistochemistry. The most abundant mRNA transcripts found in a hybridoma cell line did not necessarily encode the antibody chains providing the correct specificity. Consequently, when cloning antibody genes, functional validation of all possible VH and VL combinations is required to identify those with the highest affinity and lowest cross-reactivity. These findings, reflecting the current state of hybridomas used in research, reiterate the importance of using sequence-defined recombinant antibodies for research or diagnostic use.

Published
2018

2. An unanticipated early function of DEAD-box ATPase Prp28 during commitment to splicing is modulated by U5 snRNP protein Prp8

Author

Price, Argenta M, Görnemann, Janina, Guthrie, Christine, and Brow, David A

Subjects
Biochemistry and Cell Biology, Biological Sciences, Genetics, 1.1 Normal biological development and functioning, 2.1 Biological and endogenous factors, Aetiology, Underpinning research, Generic health relevance, Adenosine Triphosphate, Alternative Splicing, Amino Acid Sequence, Amino Acid Substitution, DEAD-box RNA Helicases, Models, Molecular, Molecular Sequence Data, Protein Multimerization, RNA, Small Nuclear, Ribonucleoprotein, U4-U6 Small Nuclear, Ribonucleoprotein, U5 Small Nuclear, Saccharomyces cerevisiae, Saccharomyces cerevisiae Proteins, Sequence Homology, Amino Acid, Spliceosomes, pre-mRNA splicing, Prp28, Prp8, commitment complex, pre-spliceosome, Developmental Biology, Biochemistry and cell biology
Abstract

The stepwise assembly of the highly dynamic spliceosome is guided by RNA-dependent ATPases of the DEAD-box family, whose regulation is poorly understood. In the canonical assembly model, the U4/U6.U5 triple snRNP binds only after joining of the U1 and, subsequently, U2 snRNPs to the intron-containing pre-mRNA. Catalytic activation requires the exchange of U6 for U1 snRNA at the 5' splice site, which is promoted by the DEAD-box protein Prp28. Because Prp8, an integral U5 snRNP protein, is thought to be a central regulator of DEAD-box proteins, we conducted a targeted search in Prp8 for cold-insensitive suppressors of a cold-sensitive Prp28 mutant, prp28-1. We identified a cluster of suppressor mutations in an N-terminal bromodomain-like sequence of Prp8. To identify the precise defect in prp28-1 strains that is suppressed by the Prp8 alleles, we analyzed spliceosome assembly in vivo and in vitro. Surprisingly, in the prp28-1 strain, we observed a block not only to spliceosome activation but also to one of the earliest steps of assembly, formation of the ATP-independent commitment complex 2 (CC2). The Prp8 suppressor partially corrected both the early assembly and later activation defects of prp28-1, supporting a role for this U5 snRNP protein in both the ATP-independent and ATP-dependent functions of Prp28. We conclude that the U5 snRNP has a role in the earliest events of assembly, prior to its stable incorporation into the spliceosome.

Published
2014

8. When monoclonal antibodies are not monospecific: Hybridomas frequently express additional functional variable regions.

Author

Bradbury, Andrew, Bradbury, Andrew, Trinklein, Nathan, Thie, Holger, Wilkinson, Ian, Tandon, Atul, Anderson, Stephen, Bladen, Catherine, Jones, Brittany, Aldred, Shelley, Bestagno, Marco, Burrone, Oscar, Maynard, Jennifer, Ferrara, Fortunato, Görnemann, Janina, Glanville, Jacob, Wolf, Philipp, Frenzel, Andre, Wong, Julin, Koh, Xin, Eng, Hui-Yan, Lane, David, Lefranc, Marie-Paule, Clark, Mike, Dübel, Stefan, Trimmer, James, Bradbury, Andrew, Bradbury, Andrew, Trinklein, Nathan, Thie, Holger, Wilkinson, Ian, Tandon, Atul, Anderson, Stephen, Bladen, Catherine, Jones, Brittany, Aldred, Shelley, Bestagno, Marco, Burrone, Oscar, Maynard, Jennifer, Ferrara, Fortunato, Görnemann, Janina, Glanville, Jacob, Wolf, Philipp, Frenzel, Andre, Wong, Julin, Koh, Xin, Eng, Hui-Yan, Lane, David, Lefranc, Marie-Paule, Clark, Mike, Dübel, Stefan, and Trimmer, James

Abstract

Monoclonal antibodies are commonly assumed to be monospecific, but anecdotal studies have reported genetic diversity in antibody heavy chain and light chain genes found within individual hybridomas. As the prevalence of such diversity has never been explored, we analyzed 185 random hybridomas, in a large multicenter dataset. The hybridomas analyzed were not biased towards those with cloning difficulties or known to have additional chains. Of the hybridomas we evaluated, 126 (68.1%) contained no additional productive chains, while the remaining 59 (31.9%) contained one or more additional productive heavy or light chains. The expression of additional chains degraded properties of the antibodies, including specificity, binding signal and/or signal-to-noise ratio, as determined by enzyme-linked immunosorbent assay and immunohistochemistry. The most abundant mRNA transcripts found in a hybridoma cell line did not necessarily encode the antibody chains providing the correct specificity. Consequently, when cloning antibody genes, functional validation of all possible VH and VL combinations is required to identify those with the highest affinity and lowest cross-reactivity. These findings, reflecting the current state of hybridomas used in research, reiterate the importance of using sequence-defined recombinant antibodies for research or diagnostic use.

Published
2018

11. Identifizierung und Charakterisierung zellulärer Proteine als Interaktionspartner des Neben-Kapsidproteins L2 Humaner Papillomviren

Author

Görnemann, Janina

Subjects
570 Life sciences
Abstract

Papillomviren sind DNA-Viren, die in einer Vielzahl von Vertebratenspezies gefunden wurden. Während die meisten Infektionen inapparent verlaufen, gibt es einige humane Papillomvirus-Typen (HPV) mit onkogenem Potential. Von besonderer Bedeutung ist dabei die Assoziation mit dem Zervixkarzinom, der zweithäufigsten Krebsart bei Frauen. Das Kapsid der Papillomviren ist aus zwei verschiedenen Kapsidproteinen aufgebaut, dem Haupt-Kapsidprotein L1 sowie dem Neben-Kapsidprotein. Die Kapsidproteine schützen nicht nur die DNA in der extrazellulären Phase des Virus und ermöglichen die Bindung des Virus an die Wirtszelle - L2 scheint auch regulatorische Funktionen zu haben. L2 spielt möglicherweise eine entscheidende Rolle bei der DNA-Verpackung und der Reifung infektiöser Virionen. In der hier vorgelegten Arbeit wurden zelluläre Interaktionspartner von L2 identifiziert. Zu diesem Zweck wurde eine humane Keratinozyten-cDNA-Bibliothek mittels des Yeast Two Hybrid-Verfahrens nach Interaktionspartnern von HPV 11 L2 durchsucht. Auf diese Weise gefundene potentielle Interaktionspartner wurden auf eine Wechselwirkung mit den L2-Proteinen anderer HPV-Typen untersucht (HPV1, HPV16). Proteine, die dabei mit mehr als einem L2-Protein interagierten, wurden auf die Bindung von HPV 16 L2 in vitro getestet und ihre subzelluläre Lokalisation analysiert. Ein mit L2 in punktartigen Kerndomänen kolokalisierendes Protein, PLINP benannt, wurde u.a. durch die Herstellung von Deletionsmutanten eingehender untersucht. Es konnte so die L2-bindende Domäne sowie der für die Lokalisation in Kerndomänen verantwortliche Bereich eingegrenzt werden. Da für BPV 1 L2 eine Lokalisation in PODs, einer ebenfalls in einem Punktmuster vorliegenden Kerndomäne, beschrieben war, wurde die Lokalisation von L2 und PLINP im Verhältnis zu PODs untersucht. Eine Assoziation dieser beiden Proteine mit PODs scheint zwar vorzuliegen, nicht aber eine ausgeprägte Kolokalisation wie zuvor für BPV 1 L2 beschrieben.

Published
2002
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14. A Role for PP1/NIPP1 in Steering Migration of Human Cancer Cells

Author

Martin-Granados, Cristina, primary, Prescott, Alan R., additional, Van Dessel, Nele, additional, Van Eynde, Aleyde, additional, Arocena, Miguel, additional, Klaska, Izabela P., additional, Görnemann, Janina, additional, Beullens, Monique, additional, Bollen, Mathieu, additional, Forrester, John V., additional, and McCaig, Colin D., additional

Published
2012
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