Your search keyword '"Mora-Jensen H"' showing total 11 results

1. Cellular origin of prognostic chromosomal aberrations in AML patients

Author

Mora-Jensen, H, Jendholm, J, Rapin, N, Andersen, M K, Roug, A S, Bagger, F O, Bullinger, L, Winther, O, Borregaard, N, Porse, B T, and Theilgaard-Mönch, K

Published

2015

2. The Bruton Tyrosine Kinase (BTK) Inhibitor Acalabrutinib Demonstrates Potent On-Target Effects and Efficacy in Two Mouse Models of Chronic Lymphocytic Leukemia.

Author

Herman SEM, Montraveta A, Niemann CU, Mora-Jensen H, Gulrajani M, Krantz F, Mantel R, Smith LL, McClanahan F, Harrington BK, Colomer D, Covey T, Byrd JC, Izumi R, Kaptein A, Ulrich R, Johnson AJ, Lannutti BJ, Wiestner A, and Woyach JA

Subjects

Adenine analogs & derivatives, Adoptive Transfer methods, Agammaglobulinaemia Tyrosine Kinase, Animals, Antineoplastic Combined Chemotherapy Protocols administration & dosage, Apoptosis drug effects, Disease Models, Animal, Humans, Leukemia, Lymphocytic, Chronic, B-Cell genetics, Leukemia, Lymphocytic, Chronic, B-Cell pathology, Mice, Mice, Transgenic, Piperidines, Protein Kinase Inhibitors administration & dosage, Protein-Tyrosine Kinases genetics, Pyrazoles administration & dosage, Pyrimidines administration & dosage, Xenograft Model Antitumor Assays, Benzamides administration & dosage, Leukemia, Lymphocytic, Chronic, B-Cell drug therapy, Protein-Tyrosine Kinases antagonists & inhibitors, Proto-Oncogene Proteins genetics, Pyrazines administration & dosage

Abstract

Purpose: Acalabrutinib (ACP-196) is a novel, potent, and highly selective Bruton tyrosine kinase (BTK) inhibitor, which binds covalently to Cys481 in the ATP-binding pocket of BTK. We sought to evaluate the antitumor effects of acalabrutinib treatment in two established mouse models of chronic lymphocytic leukemia (CLL). Experimental Design: Two distinct mouse models were used, the TCL1 adoptive transfer model where leukemic cells from Eμ-TCL1 transgenic mice are transplanted into C57BL/6 mice, and the human NSG primary CLL xenograft model. Mice received either vehicle or acalabrutinib formulated into the drinking water. Results: Utilizing biochemical assays, we demonstrate that acalabrutinib is a highly selective BTK inhibitor as compared with ibrutinib. In the human CLL NSG xenograft model, treatment with acalabrutinib demonstrated on-target effects, including decreased phosphorylation of PLCγ2, ERK, and significant inhibition of CLL cell proliferation. Furthermore, tumor burden in the spleen of the mice treated with acalabrutinib was significantly decreased compared with vehicle-treated mice. Similarly, in the TCL1 adoptive transfer model, decreased phosphorylation of BTK, PLCγ2, and S6 was observed. Most notably, treatment with acalabrutinib resulted in a significant increase in survival compared with mice receiving vehicle. Conclusions: Treatment with acalabrutinib potently inhibits BTK in vivo , leading to on-target decreases in the activation of key signaling molecules (including BTK, PLCγ2, S6, and ERK). In two complementary mouse models of CLL, acalabrutinib significantly reduced tumor burden and increased survival compared with vehicle treatment. Overall, acalabrutinib showed increased BTK selectivity compared with ibrutinib while demonstrating significant antitumor efficacy in vivo on par with ibrutinib. Clin Cancer Res; 23(11); 2831-41. ©2016 AACR ., (©2016 American Association for Cancer Research.)

Published

2017

3. Changes in Gene Expression during G-CSF-Induced Emergency Granulopoiesis in Humans.

Author

Pedersen CC, Borup R, Fischer-Nielsen A, Mora-Jensen H, Fossum A, Cowland JB, and Borregaard N

Subjects

Antimicrobial Cationic Peptides deficiency, Antimicrobial Cationic Peptides genetics, Apoptosis immunology, Cell Movement, Cytokines immunology, Cytokines metabolism, Healthy Volunteers, Humans, Microarray Analysis, Neutrophils drug effects, Recombinant Proteins immunology, Cathelicidins, Gene Expression, Granulocyte Colony-Stimulating Factor pharmacology, Leukopoiesis genetics, Neutrophils physiology

Abstract

Emergency granulopoiesis refers to the increased production of neutrophils in bone marrow and their release into circulation induced by severe infection. Several studies point to a critical role for G-CSF as the main mediator of emergency granulopoiesis. However, the consequences of G-CSF stimulation on the transcriptome of neutrophils and their precursors have not yet been investigated in humans. In this work, we examine the changes in mRNA expression induced by administration of G-CSF in vivo, as a model of emergency granulopoiesis in humans. Blood samples were collected from healthy individuals after 5 d of G-CSF administration. Neutrophil precursors were sorted into discrete stages of maturation by flow cytometry, and RNA was subjected to microarray analysis. mRNA levels were compared with previously published expression levels in corresponding populations of neutrophil precursors isolated from bone marrow of untreated, healthy individuals. One thousand one hundred and ten mRNAs were differentially expressed >2-fold throughout terminal granulopoiesis. Major changes were seen in pathways involved in apoptosis, cytokine signaling, and TLR pathways. In addition, G-CSF treatment reduced the levels of four of five measured granule proteins in mature neutrophils, including the proantibacterial protein hCAP-18, which was completely deficient in neutrophils from G-CSF-treated donors. These results indicate that multiple biological processes are altered to satisfy the increased demand for neutrophils during G-CSF-induced emergency granulopoiesis in humans., (Copyright © 2016 by The American Association of Immunologists, Inc.)

Published

2016

4. Differential expression of granulopoiesis related genes in neutrophil subsets distinguished by membrane expression of CD177.

Author

Hu N, Mora-Jensen H, Theilgaard-Mönch K, Doornbos-van der Meer B, Huitema MG, Stegeman CA, Heeringa P, Kallenberg CG, and Westra J

Subjects

Adult, Aged, Cell Membrane metabolism, Female, GPI-Linked Proteins genetics, GPI-Linked Proteins metabolism, Gene Expression Regulation, Humans, Isoantigens genetics, Male, Middle Aged, Neutrophils cytology, Oligonucleotide Array Sequence Analysis, Receptors, Cell Surface genetics, Anti-Neutrophil Cytoplasmic Antibody-Associated Vasculitis metabolism, Gene Expression Profiling methods, Gene Regulatory Networks, Isoantigens metabolism, Neutrophils metabolism, Receptors, Cell Surface metabolism

Abstract

Objective: Differential gene expression in CD177+ and CD177- neutrophils was investigated, in order to detect possible differences in neutrophil function which could be related to the pathogenesis of ANCA-associated Vasculitides (AAV)., Methods: Neutrophils were isolated from healthy controls (HC) with high, negative or bimodal CD177 expression, and sorted into CD177+ and CD177- subpopulations. Total RNA was screened for expression of 24,000 probes with Illumina Ref-8 Beadchips. Genes showing differential expression between CD177+ and CD177- subsets in microarray analysis were re-assessed using quantitative-PCR. CD177 expression on neutrophil precursors in bone marrow was analyzed using quantitative PCR and flowcytometry., Results: The proportion of CD177+ cells increased during neutrophil maturation in bone marrow. Fold change analysis of gene expression profile of sorted CD177+ and CD177- neutrophils resulted in 14 genes with fold change (fc) >3 difference in expression. Interestingly, 10 of these genes have been reported to change significantly in expression during neutrophil maturation, and most of these genes were granule protein (GP) coding genes. mRNA expression levels measured by RT-PCR of a number of these GP, and of PR3 and MPO were higher in the CD177- neutrophil subset in HC, however, particular granule protein amounts were comparable between CD177+ and CD177- neutrophil subsets. AAV patients had higher amounts of CD177+ neutrophils, but contrary to neutrophils from HC expression of GP-genes was increased, possibly due to activation., Conclusion: The neutrophil population can be distinguished by membrane expression of CD177 into subsets that are different in expression of GP mRNA but not in GP protein production. GP gene expression is also elevated in AAV patients, which is not explained by skewed distribution of CD177+ and CD177- subsets but may be associated with neutrophil activation during on-going inflammation.

Published

2014

5. miRNA-130a regulates C/EBP-ε expression during granulopoiesis.

Author

Larsen MT, Häger M, Glenthøj A, Asmar F, Clemmensen SN, Mora-Jensen H, Borregaard N, and Cowland JB

Subjects

Animals, Cell Differentiation genetics, Cells, Cultured, Gene Expression Regulation, Granulocyte Precursor Cells physiology, HEK293 Cells, Humans, Mice, Mice, Inbred C57BL, Mice, Knockout, NIH 3T3 Cells, CCAAT-Enhancer-Binding Proteins genetics, Granulocytes physiology, Leukopoiesis genetics, MicroRNAs physiology

Abstract

CCAAT/enhancer binding protein-ε (C/EBP-ε) is considered a master transcription factor regulating terminal neutrophil maturation. It is essential for expression of secondary granule proteins, but it also regulates proliferation, cell cycle, and maturation during granulopoiesis. Cebpe(-/-) mice have incomplete granulocytic differentiation and increased sensitivity toward bacterial infections. The amount of C/EBP-ε messenger RNA (mRNA) increases with maturation from myeloblasts with peak level in myelocytes (MC)/metamyelocytes (MM), when the cells stop proliferating followed by a decline in more mature cells. In contrast, C/EBP-ε protein is virtually detectable only in the MC/MM population, indicating that expression in more immature cells could be inhibited by microRNAs (miRNAs). We found that miRNA-130a (miR-130a) regulates C/EBP-ε protein expression in both murine and human granulocytic precursors. Overexpression of miR-130a in a murine cell line downregulated C/EBP-ε protein and lactoferrin (Ltf), cathelicidin antimicrobial protein (Camp), and lipocalin-2 (Lcn2) mRNA expression giving rise to cells with a more immature phenotype, as seen in the Cebpe(-/-) mouse. Introduction of a C/EBP-ε mRNA without target site for miR-130a restored both C/EBP-ε production, expression of Camp and Lcn2, and resulted in the cells having a more mature phenotype. We conclude that miR-130a is important for the regulation of the timed expression of C/EBP-ε during granulopoiesis.

Published

2014

6. Comparing cancer vs normal gene expression profiles identifies new disease entities and common transcriptional programs in AML patients.

Author

Rapin N, Bagger FO, Jendholm J, Mora-Jensen H, Krogh A, Kohlmann A, Thiede C, Borregaard N, Bullinger L, Winther O, Theilgaard-Mönch K, and Porse BT

Subjects

Blotting, Western, Case-Control Studies, Follow-Up Studies, Gene Expression Profiling, Humans, Leukemia, Myeloid, Acute pathology, Oligonucleotide Array Sequence Analysis, Prognosis, RNA, Messenger genetics, Real-Time Polymerase Chain Reaction, Reverse Transcriptase Polymerase Chain Reaction, Survival Rate, Biomarkers, Tumor genetics, Hematopoietic Stem Cells metabolism, Leukemia, Myeloid, Acute genetics

Abstract

Gene expression profiling has been used extensively to characterize cancer, identify novel subtypes, and improve patient stratification. However, it has largely failed to identify transcriptional programs that differ between cancer and corresponding normal cells and has not been efficient in identifying expression changes fundamental to disease etiology. Here we present a method that facilitates the comparison of any cancer sample to its nearest normal cellular counterpart, using acute myeloid leukemia (AML) as a model. We first generated a gene expression-based landscape of the normal hematopoietic hierarchy, using expression profiles from normal stem/progenitor cells, and next mapped the AML patient samples to this landscape. This allowed us to identify the closest normal counterpart of individual AML samples and determine gene expression changes between cancer and normal. We find the cancer vs normal method (CvN method) to be superior to conventional methods in stratifying AML patients with aberrant karyotype and in identifying common aberrant transcriptional programs with potential importance for AML etiology. Moreover, the CvN method uncovered a novel poor-outcome subtype of normal-karyotype AML, which allowed for the generation of a highly prognostic survival signature. Collectively, our CvN method holds great potential as a tool for the analysis of gene expression profiles of cancer patients.

Published

2014

7. Olfactomedin 4 defines a subset of human neutrophils.

Author

Clemmensen SN, Bohr CT, Rørvig S, Glenthøj A, Mora-Jensen H, Cramer EP, Jacobsen LC, Larsen MT, Cowland JB, Tanassi JT, Heegaard NH, Wren JD, Silahtaroglu AN, and Borregaard N

Subjects

Bone Marrow Cells drug effects, Bone Marrow Cells metabolism, Cell Differentiation genetics, Granulocyte Colony-Stimulating Factor genetics, Granulocyte Colony-Stimulating Factor pharmacology, Humans, Myeloid Cells drug effects, Myeloid Cells metabolism, Neutrophils drug effects, Protein Transport physiology, RNA, Messenger metabolism, Granulocyte Colony-Stimulating Factor metabolism, Neutrophils classification, Neutrophils metabolism

Abstract

OLFM4 was identified initially as a gene highly induced in myeloid stem cells by G-CSF treatment. A bioinformatics method using a global meta-analysis of microarray data predicted that OLFM4 would be associated with specific granules in human neutrophils. Subcellular fractionation of peripheral blood neutrophils demonstrated complete colocalization of OLFM4 with the specific granule protein NGAL, and stimulation of neutrophils with PMA resulted in corelease of NGAL and OLFM4, proving that OLFM4 is a genuine constituent of neutrophil-specific granules. In accordance with this, OLFM4 mRNA peaked at the MY/MM stage of maturation. OLFM4 was, however, present in only 20-25% of peripheral blood neutrophils, as determined by immunocytochemistry and flow cytometry, whereas mRNA for OLFM4 was present in all MY/MM, indicating post-transcriptional regulation as a basis for the heterogeneous expression of OLFM4 protein.

Published

2012

8. Technical advance: immunophenotypical characterization of human neutrophil differentiation.

Author

Mora-Jensen H, Jendholm J, Fossum A, Porse B, Borregaard N, and Theilgaard-Mönch K

Subjects

Blotting, Western, Bone Marrow metabolism, Cell Line, Cell Separation, Flow Cytometry, Granulocyte Precursor Cells cytology, Granulocyte Precursor Cells immunology, Granulocyte Precursor Cells metabolism, Granulocytes cytology, Granulocytes immunology, Granulocytes metabolism, Humans, Immunoenzyme Techniques, Myeloid Cells cytology, Myeloid Cells immunology, Myeloid Cells metabolism, Myeloid Progenitor Cells cytology, Myeloid Progenitor Cells immunology, Myeloid Progenitor Cells metabolism, Neutrophils metabolism, RNA, Messenger genetics, Reverse Transcriptase Polymerase Chain Reaction, Cell Differentiation, Immunophenotyping, Neutrophils cytology, Neutrophils immunology

Abstract

The current study reports a flow cytometry-based protocol for the prospective purification of human BM populations representing six successive stages of terminal neutrophil differentiation, including early promyelocytes and late promyelocytes, myelocytes, metamyelocytes, band cells, and PMN neutrophilic granulocytes. Validation experiments revealed a high purity of each bone marrow population and biological meaningful expression profiles for marker genes of neutrophil differentiation at a hitherto unprecedented resolution. Hence, the present protocol should be useful for studying neutrophil differentiation in vivo in the human setting and constitutes an important alternative to models that are based on in vitro differentiation of myeloid cell lines and HPCs.

Published

2011

9. Bortezomib resistance in mantle cell lymphoma is associated with plasmacytic differentiation.

Author

Pérez-Galán P, Mora-Jensen H, Weniger MA, Shaffer AL 3rd, Rizzatti EG, Chapman CM, Mo CC, Stennett LS, Rader C, Liu P, Raghavachari N, Stetler-Stevenson M, Yuan C, Pittaluga S, Maric I, Dunleavy KM, Wilson WH, Staudt LM, and Wiestner A

Subjects

ADP-ribosyl Cyclase 1 biosynthesis, Aged, Blotting, Western, Bortezomib, Cell Differentiation, Cell Line, Tumor, Cell Separation, Enzyme-Linked Immunosorbent Assay, Female, Flow Cytometry, Gene Expression Profiling, Humans, Interferon Regulatory Factors biosynthesis, Lymphoma, Mantle-Cell genetics, Lymphoma, Mantle-Cell metabolism, Male, Middle Aged, Oligonucleotide Array Sequence Analysis, Proteasome Endopeptidase Complex drug effects, Proteasome Endopeptidase Complex genetics, Proteasome Endopeptidase Complex metabolism, Antineoplastic Agents pharmacology, Boronic Acids pharmacology, Drug Resistance, Neoplasm physiology, Lymphoma, Mantle-Cell drug therapy, Plasma Cells pathology, Pyrazines pharmacology

Abstract

Bortezomib induces remissions in 30%-50% of patients with relapsed mantle cell lymphoma (MCL). Conversely, more than half of patients' tumors are intrinsically resistant to bortezomib. The molecular mechanism of resistance has not been defined. We generated a model of bortezomib-adapted subclones of the MCL cell lines JEKO and HBL2 that were 40- to 80-fold less sensitive to bortezomib than the parental cells. Acquisition of bortezomib resistance was gradual and reversible. Bortezomib-adapted subclones showed increased proteasome activity and tolerated lower proteasome capacity than the parental lines. Using gene expression profiling, we discovered that bortezomib resistance was associated with plasmacytic differentiation, including up-regulation of IRF4 and CD38 and expression of CD138. In contrast to plasma cells, plasmacytic MCL cells did not increase immunoglobulin secretion. Intrinsically bortezomib-resistant MCL cell lines and primary tumor cells from MCL patients with inferior clinical response to bortezomib also expressed plasmacytic features. Knockdown of IRF4 was toxic for the subset of MCL cells with plasmacytic differentiation, but only slightly sensitized cells to bortezomib. We conclude that plasmacytic differentiation in the absence of an increased secretory load can enable cells to withstand the stress of proteasome inhibition. Expression of CD38 and IRF4 could serve as markers of bortezomib resistance in MCL. This study has been registered at http://clinicaltrials.gov as NCT00131976.

Published

2011

10. ERAD inhibitors integrate ER stress with an epigenetic mechanism to activate BH3-only protein NOXA in cancer cells.

Author

Wang Q, Mora-Jensen H, Weniger MA, Perez-Galan P, Wolford C, Hai T, Ron D, Chen W, Trenkle W, Wiestner A, and Ye Y

Subjects

Adaptor Proteins, Signal Transducing, Antineoplastic Agents pharmacology, Boronic Acids pharmacology, Bortezomib, Cell Line, Cell Line, Tumor, HeLa Cells, Humans, Hydrazones metabolism, Hydroxyurea analogs & derivatives, Hydroxyurea metabolism, Neoplasms metabolism, Pyrazines pharmacology, Transcription, Genetic, Adaptor Proteins, Vesicular Transport metabolism, Endoplasmic Reticulum metabolism, Epigenesis, Genetic, Gene Expression Regulation, Neoplastic, Proteasome Endopeptidase Complex chemistry, Ubiquitin chemistry

Abstract

The ubiquitin-proteasome system has recently emerged as a major target for drug development in cancer therapy. The proteasome inhibitor bortezomib has clinical activity in multiple myeloma and mantle cell lymphoma. Here we report that Eeyarestatin I (EerI), a chemical inhibitor that blocks endoplasmic reticulum (ER)-associated protein degradation, has antitumor and biologic activities similar to bortezomib and can synergize with bortezomib. Like bortezomib, EerI-induced cytotoxicity requires the up-regulation of the Bcl-2 homology3 (BH3)-only pro-apoptotic protein NOXA. We further demonstrate that both EerI and bortezomib activate NOXA via an unanticipated mechanism that requires cooperation between two processes. First, these agents elicit an integrated stress response program at the ER to activate the CREB/ATF transcription factors ATF3 and ATF4. We show that ATF3 and ATF4 form a complex capable of binding to the NOXA promoter, which is required for NOXA activation. Second, EerI and bortezomib also block ubiquitination of histone H2A to relieve its inhibition on NOXA transcription. Our results identify a class of anticancer agents that integrate ER stress response with an epigenetic mechanism to induce cell death.

Published

2009

11. Noxa mediates bortezomib induced apoptosis in both sensitive and intrinsically resistant mantle cell lymphoma cells and this effect is independent of constitutive activity of the AKT and NF-kappaB pathways.

Author

Rizzatti EG, Mora-Jensen H, Weniger MA, Gibellini F, Lee E, Daibata M, Lai R, and Wiestner A

Subjects

Bortezomib, Cell Line, Tumor, Dose-Response Relationship, Drug, Humans, Lymphoma, Mantle-Cell drug therapy, Proto-Oncogene Proteins c-bcl-2 genetics, Signal Transduction, Up-Regulation, Apoptosis drug effects, Boronic Acids pharmacology, Lymphoma, Mantle-Cell pathology, NF-kappa B metabolism, Proto-Oncogene Proteins c-akt metabolism, Proto-Oncogene Proteins c-bcl-2 physiology, Pyrazines pharmacology

Abstract

Bortezomib is more active against mantle cell lymphoma (MCL) than against most other lymphoma subtypes. Nevertheless, up to half of patients with MCL have bortezomib resistant disease. Factors contributing to intrinsic resistance to bortezomib have not been determined. Here we used a panel of eight bortezomib sensitive (median IC(50) 5.9 nM) and three relatively bortezomib resistant cell lines (median IC(50) 12.9 nM) to investigate differences in tumor biology that could determine sensitivity to bortezomib. Bortezomib effectively inhibited high baseline proteasome activity and induced a comparable degree of proteasome inhibition in both sensitive and resistant cells. At 10 nM, bortezomib induced the proapoptotic BH3-only protein Noxa in sensitive but not resistant cells. At higher concentrations of bortezomib, however, Noxa was also upregulated in resistant cells and this effect was sufficient to induce apoptosis. Silencing of Noxa with siRNA rescued these cells from apoptosis, arguing against a defect in Noxa regulation or function as the basis of bortezomib resistance. Bortezomib was equally effective against cells with high and low constitutive NF-kappaB signaling. Also, sensitive and resistant MCL cell lines showed comparable activation of the AKT pathway. We conclude that bortezomib can overcome classic mechanisms of resistance to apoptosis and that determinants of bortezomib sensitivity in MCL are due to differences in signaling or stress pathways upstream of Noxa.

Published

2008