Bmx Tyrosine Kinase Has a Redundant Function Downstream of Angiopoietin and Vascular Endothelial Growth Factor Receptors in Arterial Endothelium

doi:10.1128/MCB.21.14.4647-4655.2001

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Rajantie, I.
	Articles by Alitalo, K.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Rajantie, I.
	Articles by Alitalo, K.

Previous Article | Next Article

Molecular and Cellular Biology, July 2001, p. 4647-4655, Vol. 21, No. 14
0270-7306/01/$04.00+0 DOI: 10.1128/MCB.21.14.4647-4655.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Bmx Tyrosine Kinase Has a Redundant Function Downstream of Angiopoietin and Vascular Endothelial Growth Factor Receptors in Arterial Endothelium

Iiro Rajantie,¹ Niklas Ekman,¹ Kristiina Iljin,¹ Elena Arighi,¹ Yuji Gunji,¹ Jaakko Kaukonen,² Aarno Palotie,² Mieke Dewerchin,³ Peter Carmeliet,³ and Kari Alitalo¹^,^*

Molecular/Cancer Biology Laboratory, Haartman Institute and Biomedicum Helsinki,¹ and Department of Clinical Chemistry and Helsinki University Hospital,² 00014 University of Helsinki, Finland, and Center for Transgene Technology and Gene Therapy, Flanders Interuniversity Institute for Biotechnology, Campus Gasthuisberg, University of Leuven, Leuven B-3000, Belgium³

Received 14 February 2001/Returned for modification 23 March 2001/Accepted 25 April 2001

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

The Bmx gene, a member of the Tec tyrosine kinase gene family, is known to be expressed in subsets of hematopoietic and endothelialcells. In this study, mice were generated in which the first codingexon of the Bmx gene was replaced with the lacZ reporter geneby a knock-in strategy. The homozygous mice lacking Bmx activitywere fertile and had a normal life span without an obvious phenotype.Staining of their tissues using $beta$ -galactosidase substrate to assessthe sites of Bmx expression revealed strong signals in the endothelialcells of large arteries and in the endocardium starting betweendays 10.5 and 12.5 of embryogenesis and continuing in adult mice,while the venular endothelium showed a weak signal only in thesuperior and inferior venae cavae. Of the five known endothelialreceptor tyrosine kinases tested, activated Tie-2 induced tyrosylphosphorylation of the Bmx protein and both Tie-2 and vascularendothelial growth factor receptor 1 (VEGFR-1) stimulated Bmxtyrosine kinase activity. Thus, the Bmx tyrosine kinase has aredundant role in arterial endothelial signal transduction downstreamof the Tie-2 and VEGFR-1 growth factorreceptors.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Endothelial cells perform overlapping but also distinct functions in different parts of the cardiovascular system (28).The pericellular environment of venular and arterial endothelialcells differs primarily in the relative oxygen content of theblood, blood pressure, fluid shear forces, and periendothelialmatrix and smooth muscle structures. The arterial endotheliumis required to withstand an exceptionally strong stress causedby pulsatile blood flow. It also has a role in the control ofsmooth muscle cell tone in the vessel wall and thus of blood pressure(22). Dysfunction of the endothelium contributes to pathologicalconditions of the arterial wall, such as atherosclerosis (23).Recently, molecular cloning has increased our knowledge of geneexpression specific for the arterial endothelial cells and ofthe mechanisms leading to distinct properties of the arteriesandveins.

Tyrosine kinases (TKs) play a central role in signal transduction in endothelial cells. They activate growth and differentiationsignal cascades through phosphorylation of cellular proteins (8,27, 31). For example, the EphB4 receptor TK and its ligandephrin B2 are considered to be responsible for signaling earlyarteriovenous differentiation (1, 39). Also, the recentlyreported expression of Dll4, a member of the Delta family of Notchligands, in arterial endothelial cells indicates the existenceof additional arterial endothelium-specific signal transductioncascades (33). In endothelial cells, TKs activate pathways resultingin the expression of proteins and factors which function as regulatorsof vessel tone (e.g., nitric oxide and endothelin 1), adhesionmolecules (e.g., vascular cell adhesion molecule 1), or chemoattractants(e.g., monocyte chemoattractant protein 1) (for reviews, see reference14). Mechanical stress activates a number of signaling pathwaysleading to changes in the conformation of arterial endothelialcells and in their interactions with pericellular matrix, forexample, in focal adhesions (9, 38).

Bmx is a member of the Tec family of TKs, which also includes the Tec, Btk, Itk/Tsk/Emt, and Rlk/Txk kinases (24). The Teckinases are expressed mainly in hematopoietic cells, where theytransduce growth and differentiation signals from a variety ofcytokine and antigen receptors. For example, the Tec TK occursin most hematopoietic cells, while Btk is expressed selectivelyat certain stages of lymphocyte development and in the myeloidcell lineage (for reviews, see reference 41). Like the othermembers of the Tec family, Bmx is expressed in the myeloid hematopoieticcell lineage (15, 40). In myeloid progenitor cells, Bmx waspreviously shown to regulate cell differentiation and maturation(4). In addition, Bmx mRNA has been detected in the endotheliumof large arteries by in situ hybridization of mouse embryos (5).

In this study, we have replaced the first coding exon of the Bmx gene with the lacZ gene encoding $beta$ -galactosidase. While theloss of Bmx function gave no obvious phenotype, the model alloweda detailed study of Bmx expression in arterial endothelial cellsof fetal and adult tissues. Based on this analysis, we also showthat the endothelium-specific TK receptors Tie-2/Tek and vascularendothelial growth factor receptor 1 (VEGFR-1) are upstream regulatorsof Bmx in the arterialendothelium.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Construction of the targeting vector. Mouse 129Sv genomic clones flanking the first coding exon of the Bmx gene were used to generate the targeting vector pPNT-Bmx-LacZ.A 10.5-kb BamHI-KpnI fragment containing the 5' flanking sequenceof the first coding exon was fused to the bacterial lacZ geneand blunt end cloned as the 5' arm of the pPNT targeting vectordescribed previously (32). A 1.8-kb EcoRI-ClaI fragment 3' ofthe first coding exon was blunt end cloned into the pPNT vectorand used as the 3' homology arm. The targeting construct replacesthe exon containing the translation initiation codon, therebyinactivating thegene.

Generation and genotyping of the Bmx^/ mice. Electroporation of embryonic stem (ES) cells and generation of chimeric mice transmitting the mutation in the germ line werefollowed by mating of heterozygous and homozygous knockout mice(2). To identify Bmx-deficient mice, Southern blot analysiswas carried out using genomic DNA purified from tail biopsy specimensof 4-week-old mice. The mouse strain used was DBA/2. All experimentsusing the mice were approved by the Helsinki University LaboratoryAnimal Committee. Ten male and ten female mice were used withidenticalresults.

RNA isolation and analysis. Total RNA from mouse bone marrow was extracted using the RNAeasy kit (Qiagen) according to the manufacturer's instructions.The reverse transcription (RT) reaction was carried out with 0.5µg of total RNA, using the Omniscript RT Kit (Qiagen) and randomhexanucleotide primers in a total volume of 20 µl. Following theRT reaction, the Bmx cDNA was PCR amplified from 4 µl of RT productusing 5'-AACATACGCTATATTCCA-3' and 5'-GCATGCAGATTTTCCTCT-3' asprimers for 25 cycles. The reaction conditions were 94°C for 40s, 49°C for 30 s, and 72°C for 72 s. The LacZ cDNA was amplifiedfor 15 cycles using 5'-GCTGCATAAACCGACTACAC-3'and 5'-TTCACCCTGCCATAAAGAAAC-3'as primers with the following conditions: 94°C for 30 s, 56°Cfor 30 s, and 72°C for 30 s. Both amplifications were carriedout using Dynazyme (Finnzymes) polymerase in a total volume of50 µl. Following the amplification, 10 µl of each PCR mixturewas electrophoresed in a 1.5% agarose gel and Southern blottedonto a Hybond N⁺ (Amersham Pharmacia Biotech) nylon filter under alkaline conditions.The filters were hybridized with Bmx or LacZ cDNA probes usingQuickHyb (Stratagene) solution and stringent washingconditions.

$beta$ -Galactosidase staining of tissues. Embryos and whole-mount adult tissues were fixed in 0.2% glutaraldehyde-2 mM MgCl₂-5 mM EGTA in 100 mM phosphate buffer atroom temperature for 15 to 30 min. The tissues were then washedat room temperature in wash buffer (2 mM MgCl₂, 0.01% deoxycholate,0.02% Nonidet P-40 in 100 mM phosphate buffer) and incubated in1-mg/ml X-Gal reaction mixture [1 mg of 5-bromo-4-chloro-3-indolyl- $beta$ -galactosidase/ml,5 mmol of K₃Fe(CN)₆/liter, 5 mmol of K₄Fe(CN)₆/liter in wash buffer]at 37°C overnight. After staining, the samples were incubatedin wash buffer at 4°C, transferred into 4% paraformaldehyde inphosphate-buffered saline (PBS), and fixed at 4°C overnight. Thetissues were dehydrated through graded ethanols and embedded inparaffin. Sections were cut at 7 µm, mounted onto glass slides,dewaxed, and stained with nuclear fastred.

Immunostaining. Tissues were fixed in 4% paraformaldehyde at 4°C overnight, dehydrated, and embedded in paraffin. Five-micrometer-thick paraffinsections were incubated for 20 min in 250 µg of trypsin/ml at37°C and stained with endothelial-cell-specific platelet endothelialcell adhesion molecule 1 antibodies (Abs) (1:1,000; Pharmingen)using the Tyramide signal amplification (TSA) kit (NEN Life Sciences).For Tie-2 and smooth muscle $beta$ -actin (SMA) staining, the sectionswere heated in a microwave oven in 10 mM sodium citrate, blockedaccording to the manufacturer's instructions, and incubated withrabbit polyclonal anti-Tie-2 (1:500; Santa Cruz) and monoclonalanti-SMA (1:100, alkaline phosphatase conjugated; Sigma), respectively.The Tie-2-stained sections were processed further using the TSAkit, and the SMA-stained sections were processed using the AlkalinePhosphatase Substrate II kit (Vector Laboratories). The slideswere counterstained inhematoxylin.

Lectin staining of blood vessels. Lectin staining was used to visualize blood vessels in whole mounts of tissue as described previously (36). BiotinylatedLycopersicon esculentum lectin (100 µl of a 1-mg/ml solution;Sigma catalog no. B-1175) was injected intravenously via the femoralvein into anesthetized mice and allowed to circulate for 2 min.The mice were then sacrificed, and the tissues were fixed by intracardialperfusion with 1% paraformaldehyde-0.5% glutaraldehyde in PBS.The ears were dissected and washed with PBS, and the cartilagewas removed. Bound lectin was visualized by biotin-peroxidasestaining, and the ears were mounted on slides and examined bylightmicroscopy.

Fluorescence in situ hybridization of metaphase chromosomes. Fetal cell culture was established from a male mouse according to routine protocols (7). Part of the mouse genomic BmxDNA was identified, isolated, and cloned from a mouse 129Sv genomicDNA library in the lambda FIX II vector (Stratagene), using aPCR fragment containing human Bmx cDNA nucleotides 23 to 162 asa probe. The insert was subcloned as a SalI fragment into pBluescriptSK II (Stratagene) and labeled with digoxigenin-11-dUTP (BoehringerMannheim) according to standard procedures. The single-color metaphasefluorescence in situ hybridization was performed and analyzedessentially as described previously (13).

Cell culture, growth factor stimulation, DNA constructs, and cell transfections. 293T cells were grown in Dulbecco's modified Eagle's medium containing 10% fetal calf serum, glutamine, and antibiotics. Humandermal microvascular endothelial (HDME) cells, obtained from PromoCell, were grown in MV low-serum endothelial cell growth medium(Promo Cell) supplemented with the endothelial cell supplementmix provided by Promo Cell. The HDME cells were starved in serum-and growth factor-free media containing 0.2% bovine serum albuminfor 45 h prior to 20-min stimulation with either angiopoietin-1(Ang-1)-conditioned medium produced by transfected 293T cellsor 100 ng of hVEGF165 (R&D Systems)/ml. The Ang-1 expression plasmidwas produced by PCR amplification of human Ang-1 (21), followedby cloning into the SignalpIG vector (Ingenius; R&D Systems).All other DNA constructs used have been previously described (4,19). The 293T cells were transiently transfected using a calciumphosphate transfection kit (GIBCO Life Technologies) accordingto the manufacturer'sinstructions.

Abs, immunoblotting, and in vitro Bmx kinase assay. The monoclonal antihemagglutinin (anti-HA) epitope and anti-Bmx Abs were obtained from Berkeley Antibody Company and TransductionLaboratories, respectively, while the phosphotyrosine-specificmouse monoclonal Ab 4G10 was from Upstate Biotechnology. Abs tothe endothelial cell receptors studied were the following: forTie-1, MII (rabbit polyclonal anti-human Tie-1) (25); for Tie-2,goat polyclonal anti-human Tie-2 (R&D Systems); for VEGFR-1, P1-3rabbit polyclonal anti-human VEGFR-1 (a kind gift from MasabumiShibuya); for VEGFR-2, RS2 (rabbit polyclonal anti-human-VEGFR-2;a kind gift from Lena Claesson-Welsh); and for VEGFR-3, 9D9 mousemonoclonal anti-human VEGFR-3 (12). For immunoprecipitation,cells were lysed in TKB lysis buffer (1% NP-40, 20 mM Tris-HCl[pH 7.5], 150 mM NaCl, 5 mM EDTA, 10% glycerol) supplemented withaprotinin, leupeptin, phenylmethylsulfonyl fluoride, and sodiumvanadate. Immunoprecipitation was carried out from equal amountsof cell lysates by adding specific Abs and protein A-Sepharose(Amersham Pharmacia Biotech AB) or protein G-Sepharose (AmershamPharmacia Biotech AB) and incubating for 1 h. The Bmx in vitrokinase assays were done as described previously (4). Briefly,the immunoprecipitates were washed twice with lysis buffer, oncewith wash buffer (150 mM NaCl, 20 mM HEPES, pH 7.4), and twicewith kinase assay buffer (10 mM HEPES [pH 7.4], 5 mM MnCl₂) andresuspended in 25 µl of reaction buffer (kinase assay buffer,10 µM unlabeled ATP, 5 µCi of $gamma$ -ATP). The kinase reactions werecarried out at 30°C for 10 min and stopped by adding an equalvolume of 2× reducing Laemmli buffer. For Western blotting, theimmunoprecipitates were washed four times with the lysis bufferfollowed by elution with the Laemmli buffer and separation insodium dodecyl sulfate-7.5% polyacrylamide gels. The proteinswere transferred to a nitrocellulose membrane and detected usingspecific primary Abs, biotinylated anti-mouse or anti-rabbit secondaryAbs (Dako A/S), and streptavidin-biotin-horseradish peroxidaseconjugate (Amersham Life Science) followed by detection by theECL method (Amersham LifeScience).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Generation of mice expressing the lacZ gene under the mouse Bmx promoter. In order to study the expression pattern of the Bmx gene in embryos and adult tissues, it was replaced with the bacteriallacZ gene by gene targeting of ES cells. The exon encoding thetranslation start codon of Bmx was exchanged with the lacZ gene,placing the latter under the control of the Bmx promoter. R1 EScells were electroporated with the targeting vector describedin Materials and Methods. Several double-resistant drug-selectedcell lines were obtained where homologous recombination had occurred,as evidenced by Southern blotting and hybridization of genomicDNA using both internal and external probes (data not shown).Two independent cell clones were used to make aggregation chimeras,which transmitted the Bmx^lacZ allele into the germ line. For the analysis, mice derived fromtwo different aggregations were used with identical results. Theknockout strategy, as well as an example of genotyping of theoffspring using Southern blotting, is shown in Fig. 1. The knockoutmice were fertile and had a normal life span.

View larger version (15K):
[in this window]
[in a new window]

FIG. 1. Gene targeting of the mouse Bmx locus. The homologous recombination event deletes the exon coding for the translation initiation codon (exon 2, black box) and places the bacterial lacZ gene under the control of the Bmx promoter region. Schematic structures of the wt and recombinant loci and the targeting vector are shown. Open box, exon 1; E, EcoRI; B, BamHI; H, HindIII; S, SalI; X, XhoI; C, ClaI; Neo, neomycin phosphotransferase gene; HSV-TK, herpes simplex virus thymidine kinase gene; kb, kilobase pairs. Genotyping of tail biopsy specimens from 4-week-old mice was carried out by Southern blotting using the indicated fragment as a probe. Shown also are the results of RT-PCR analysis of isolated RNA from bone marrow cells derived from Bmx^LacZ/Bmx^LacZ or wt mice. The upper panel shows PCR using Bmx-specific primers, while the lower panel shows PCR using LacZ-specific primers. A faint band seen upon prolonged exposure in samples from the Bmx^LacZ/Bmx^LacZ mice corresponded to the signal obtained by a 100-fold dilution of the wt DNA and was considered insignificant (data not shown).

In order to ensure that no Bmx mRNA was produced in the knockout mice, RNA from bone marrow cells from homozygous knockoutmice and wild-type (wt) controls was analyzed by RT-PCR. No BmxmRNA could be detected in the Bmx^LacZ/Bmx^LacZ mice, while a clear signal was obtained from the wt mice. Viceversa, only the knockout mice expressed LacZ mRNA. Essentiallysimilar results were also obtained using three other primer pairslocated in various regions ofBmx.

Expression of the lacZ gene in the Bmx knock-in locus. The $beta$ -galactosidase activity in the tissues of the Bmx gene-targeted mice was used to assess the sites of Bmx^lacZ expression by X-Gal staining, as explained in Materials and Methods.Most of the localization studies were carried out using mice homozygousfor the Bmx mutation, but heterozygous mice gave essentially similarresults, suggesting that deletion of the Bmx gene does not leadto significant alteration of the normal vascular development orarchitecture. No staining was obtained in 10.5-day-postconceptionembryos (E10.5; Fig. 2A). At E12.5, strong staining of the endocardiumof the heart and the endothelium of large arteries was seen inwhole-mount analysis (Fig. 2B). The aortic endothelium was positiveboth in the thoracic and in the abdominal region, and major arteriesbranching out from the aortic trunk also showed clear activityin the endothelial cells. For comparison, the Tie promoter-driven $beta$ -galactosidase expression was widely observed throughout thevascular endothelium, especially in the capillary network (Fig.2C) (see also reference 18).

View larger version (104K):
[in this window]
[in a new window]

FIG. 2. $beta$ -Galactosidase reporter staining of E10.5 (A) and E12.5 (B) Bmx^LacZ embryos and an E10.5 Tie^LacZ/Tie embryo (C). At E12.5, the strongest signals are seen in the aorta (A), internal carotid artery (ICA), vertebral artery (VA), intercostal arteries (IA), and umbilical artery (UA). An asterisk marks the heart. Bar, 500 µm.

In the E12.5 Bmx^LacZ embryos, the carotid arteries and their branches in the basal brain were positive for $beta$ -galactosidase activity,as were the vertebral arteries (Fig. 3A to C). A conspicuous signalwas also obtained from the developing venous sinus in the midlineof the roof of the midbrain (Fig. 3D). Intercostal arteries branchingfrom the descending aorta were stained but not as strongly asthe larger arteries. In general, the staining became weaker inthe more distal branches. A similar pattern of staining was obtainedin the pulmonary trunk (data not shown). The umbilical arteriesbranching from the distal part of the aorta displayed intense $beta$ -galactosidase staining in the endothelium, which continued inthe placental part, where the umbilical artery divides into smallervessels (Fig. 3E to G). The amniotic artery was also stronglypositive (Fig. 3H).

View larger version (78K):
[in this window]
[in a new window]

FIG. 3. Bmx^lacZ expression in E12.5 embryos. (A) The carotid arteries (arrows) and the heart (R, right ventricle; L, left ventricle) show $beta$ -galactosidase activity in the dissected embryo. (B) Branch point of the internal and external carotid arteries (arrow) and the internal carotid artery at the base of the brain (arrowhead, partially cut out during preparation). (C) The LacZ-positive arteries of the vascular system called the circle of Willis; the anterior part is not visible in the figure. CCeA, caudal cerebral artery; MCeA, medial cerebral artery; CCA, caudal communicating artery; RCA, rostral communicating artery; PCA, posterior communicating artery. (D) Expression in the superior sagittal dural venous sinus (arrow). (E and F) Umbilical arteries (arrows) entering the umbilical cord. The asterisk in panel F indicates the heart. (G) The umbilical artery (arrow) entering the placenta and the chorionic plate (CP). The umbilical vein (arrowhead) is negative. (H) The largest amniotic arteries (arrow) were positive. Bar, 500 µm.

At E15.5, the developing fetal skin is no longer transparent for the visualization of $beta$ -galactosidase activity, and thus,only tissue sections were studied. The major sites of expressionwere the ones identified in the whole-mount analysis of E12.5embryos, except that the staining was now also apparent in themore peripheral branches of the arteries. The endocardium of theheart was weakly stained, and a weak signal was also present inthe endothelium of the superior and inferior venae cavae closeto the sites where they enter the heart (Fig. 4A and B). The signalswere much stronger in the major arteries around the heart andalso in the peripheral arteries of the body wall. Examples ofthe arterial specificity are further illustrated in Fig. 4C andD, where the femoral artery, but not the vein and the radial artery,is stained. Also, a cross section of the umbilicus is shown inFig. 4E. However, all blood vessels of the abdominal organs werenegative in both E12.5 and E15.5 embryos (Fig. 4F). As in theE12.5 embryos, the endothelial cells lining the superior sagittaldural venous sinus were strongly positive. Remarkably, no othersites of expression could be detected.

View larger version (166K):
[in this window]
[in a new window]

FIG. 4. Staining of sections from E15.5 Bmx^LacZ embryos. (A) The endocardium of the heart ventricles (arrows). RA, right atrium; RV, the lumen of the right ventricle. (B) The endothelial cells of the aorta (A), the right pulmonary artery (RPA), and the left pulmonary artery (LPA) are also stained. In the right and left superior venae cavae (RSVC and LSVC, respectively), the endothelial lining is weakly positive. L, right lung; B, main bronchi; E, esophagus. (C) In the blood vessels of the hind limbs and tail, Bmx^lacZ expression occurs in the femoral artery (FA) and caudal artery (CA) but not in the femoral vein (FV) or lateral marginal vein (LMV) of the hind limb. GT, genital tubercle. (D) The endothelium of the radial artery (RA) is positive, whereas the cephalic vein (CV) is negative. Asterisks indicate the primordia of the metacarpal bones. (E) In the umbilical cord, Bmx^lacZ was expressed specifically in the arterial endothelium (arrow), while the venous endothelial cells (arrowhead) were negative. (F) No positive blood vessels were found in the abdominal organs, while the abdominal wall (AW) contains stained vessels (arrows). US, urogenital sinus; S, stomach; G, lumen of gut; L, left lobe of the liver. Bar, 200 µm.

Bmx^LacZ activity in adult mice. Adult mice were analyzed at 3 to 6 months postpartum. The endothelial cells of the arteries throughout the body showed strongBmx^LacZ activity, whereas capillaries were negative. For example, inthe ear, the endothelium of the arteries was positive, but sucha signal was absent from the capillaries (Fig. 5). In the brain,a signal was obtained from most vessels which were positive forSMA, indicative of their arterial nature. The capillary networkand the smallest SMA-positive arterioles were $beta$ -galactosidasenegative (Fig. 6A to C). Again, the venous endothelium was positiveonly in the superior and inferior venae cavae (Fig. 6D). In theheart, a strong signal was found in the coronary arteries andin the endothelial cells of the auricles (Fig. 6E and F).

View larger version (129K):
[in this window]
[in a new window]

FIG. 5. Whole-mount analysis of Bmx^lacZ expression in lectin-stained blood vessels of the ear. (A). In the $beta$ -galactosidase-stained ear of the lectin-perfused Bmx^LacZ mice, the endothelial cells are positive in the arteries (arrow) but negative in the veins (arrowhead). (B and D) The wt mice were negative for $beta$ -galactosidase staining. HF, hair follicle. (C) In the small arteries, the Bmx^lacZ expression was weaker and the signal was lost (arrow) in the capillary endothelium. Bar, 100 µm.

View larger version (116K):
[in this window]
[in a new window]

FIG. 6. (A to C) Bmx^lacZ expression in brain microvasculature and major vessels of adult mice. (A) Endothelial cell-specific platelet endothelial cell adhesion molecule 1 staining of the microvasculature of the cerebral cortex. (B) Simultaneous staining for SMA (brown) and $beta$ -galactosidase (blue) in cortical brain. The smooth muscle cells decorate the walls of arteries and arterioles, whereas veins (arrowhead) and capillaries are negative. Note that Bmx^lacZ signal (arrow) is present only in SMA-positive vessels, although not in the smallest ones (asterisks). (C) Overlapping expression patterns in an SMA- and X-Gal-stained section from the brain parenchyma. Symbols are as defined for panel B. (D) Weakly $beta$ -galactosidase-positive cells are present in a section from the inferior vena cava (arrowhead). (E) In whole-mount staining of the heart, a strong signal is seen in the coronary arteries (arrow, left coronary artery) and in the endothelial cells of the auricles (asterisk, left auricle). (F) In a section through the heart wall, endothelial expression of Bmx^lacZ is observed in the coronary artery (arrow) but not in the coronary vein (arrowhead). Bar, 150 µm.

In adult mice, the Bmx^lacZ gene was also expressed outside the cardiovascular system. A strong signal was present in Hassall'scorpuscles in the medulla of the thymus (Fig. 7A). The epithelioreticularcells were stained; these are of oropharyngeal origin and concentricallyarranged, with the centers of the corpuscles occasionally displayingkeratinization. Additional epithelial expression was found inthe mucous membrane of the tongue, where occasional epithelialcells in the suprabasal layer expressed $beta$ -galactosidase and someof the staining persisted in the keratinizing layer in a patch-likepattern (Fig. 7B).

View larger version (111K):
[in this window]
[in a new window]

FIG. 7. Whole-mount $beta$ -galactosidase staining of the thymus (A and B) and the tongue (C and D). (A) The Bmx^lacZ gene is expressed in a spot-like pattern in the medulla (M) of the thymus. C, cortex. (B) Histological analysis of the thymus shows positive clusters of cells (arrowheads) and blood vessels (arrows) in the medulla (M). The former are epithelial cells of the Hassall's corpuscles (inset). C, cortex. The asterisk shows the trabecula. (C) Bmx^lacZ is expressed in a patch-like pattern on the surface of the tongue. (D) Staining is strongest in certain basal cells in the mucosa and becomes weaker when the epithelial cells keratinize and move upward (inset). BC, basal cells; KC, keratinized cells. Bar, 300 µm.

Chimeric expression pattern of the X-chromosomal BmxlacZ locus. As has been previously shown for the human Bmx locus (35), the mouse Bmx locus is located in the X chromosome as detectedby in situ hybridization analysis (Fig. 8A). Because one of theX chromosomes is inactivated in a stochastic manner during embryonicdevelopment, it was of interest to compare the staining of homozygousand heterozygous Bmx^LacZ mice. As expected, a mosaiclike expression pattern was seen inheterozygous female mice, illustrated in Fig. 8B to G.

View larger version (60K):
[in this window]
[in a new window]

FIG. 8. Chromosomal localization and mosaic expression pattern of the Bmx^lacZ locus. (A) Chromosomal fluorescence in situ hybridization for the mouse Bmx gene. The Bmx gene is located in the telomeric region of the X chromosome, below band F. (B and E) The arteries on the surface of the brain cortex show a strong uniform signal in Bmx^LacZ/Bmx^LacZ mice in $beta$ -galactosidase staining. In a higher magnification, arteries (arrow, blue) appear darkly stained, whereas the veins (arrowhead, red) are visible only when filled with blood. (C and F) In the Bmx^LacZ/Bmx mice, the staining of the arterial endothelium is weaker and Bmx is detected in a mosaiclike pattern (arrow). (D and G) Bmx/Bmx control mice were negative in $beta$ -galactosidase staining. Bar, 800 µm.

The Bmx kinase activity is regulated by Tie-2 and VEGFR-1 TK receptors. Bmx expression specifically in arterial endothelial cells suggested that this TK could receive signals from endothelium-specificgrowth factor receptors. In order to investigate the ability ofendothelial cell-specific receptor TKs to phosphorylate and activateBmx, wt Bmx or "kinase-dead" (kd) Bmx was coexpressed with Tie-1,Tie-2, VEGFR-1, VEGFR-2, or VEGFR-3 in 293T cells. As can be seenfrom Fig. 9, Tie-2 coexpression increased the tyrosyl phosphorylationof both wt and catalytically inactive kd Bmx while VEGFR-1 increasedthe phosphorylation of only wt Bmx. This phosphorylation was associatedwith an increase in wt Bmx kinase activity as measured by theautophosphorylation assay. The other receptors did not affectBmx phosphorylation. The activated mutant Tie-2*, containing anarginine-to-tryptophan mutation (R849W) in the kinase domain,caused an even more potent phosphorylation of Bmx than did wtTie-2. Interestingly, this mutation has been linked to venousmalformations in humans (37).

View larger version (82K):
[in this window]
[in a new window]

FIG. 9. Bmx is activated by Tie-2 and VEGFR-1. wt Bmx (top four panels) or kd Bmx (bottom three panels) was coexpressed with the indicated endothelial cell-specific growth factor receptors in 293T cells. The cell lysates were immunoprecipitated with either anti-HA, precipitating the Bmx protein, or specific receptor Abs, followed by immunodetection with antiphosphotyrosine ( $alpha$ -pTyr) Ab or anti-HA Ab. Tyrosine-phosphorylated and activated receptors are indicated with asterisks. The immunoprecipitated Bmx was also subjected to in vitro kinase reactions as described in Materials and Methods. Note the slower-migrating (phosphorylated) isoform of Bmx in the anti-HA blot from cells expressing wt Bmx together with Tie-2* or VEGFR-1. IP, immunoprecipitation; WB, Western blotting.

Coexpression of Bmx and Tie-2 in endothelial cells. The relevance of the observed Bmx regulation by Tie-2 depends on whether these two TKs are expressed in the same cells invivo. We therefore compared the expression patterns of Bmx andTie-2 in tissue sections. Significant overlaps were detected.For example, in Fig. 10A, the Bmx^LacZ staining is shown in a branch of the aorta and the correspondingBmx-expressing endothelial cells are stained by Abs against Tie-2in Fig. 10B. We then tested cultured HDME cells for Bmx and Tie-2mRNA expression. As expected, both mRNAs were expressed at highlevels, while neither mRNA was expressed in the HEL leukemia cellline (Fig. 10C). In order to test whether the endogenous Bmx isalso activated by the Tie-2 and VEGF receptors, we stimulatedthe HDME cells with Ang-1-conditioned medium produced by transfected293T cells (Fig. 10D, lane 3) or with VEGF (lane 4). A clear increaseof Bmx kinase activity was detected following both stimulationsover that in the unstimulated cells (lane 1) or cells stimulatedwith 293T mock medium (lane 2), indicating that these receptorsactivate endogenous Bmx in cultured endothelial cells as well.

View larger version (67K):
[in this window]
[in a new window]

FIG. 10. Bmx^LacZ and Tie-2 are coexpressed in endothelial cells. (A) $beta$ -Galactosidase staining of a section from a branch of the aorta. Note the endothelial staining, shown below in higher magnification. Bars, 40 µm. (B) Immunohistochemical staining of Tie-2 in a similar section. The asterisks in panels A and B indicate the aortic lumen. (C) Northern blotting of RNA isolated from HDME cells (HDMEC) (lane 1) and HEL cells (lane 2). The filter was probed for Bmx (upper panel), followed by reprobing for Tie-2 (lower panel). (D) Serum- and growth factor-starved HDME cells were stimulated for 20 min with the indicated factors. Immunoprecipitated Bmx was subjected to in vitro kinase assay, and the activity was detected as autophosphorylation by sodium dodecyl sulfate-polyacrylamide gel electrophoresis, as has been described previously. The lower panel shows control Western blotting using anti-Bmx Abs and 15 µg of total protein per lane.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

The Bmx TK appears to be the first intracellular TK which is relatively specific for the arterial endothelium in solid tissues.It is also, to our knowledge, the first intracellular TK shownto be regulated by both the Tie-2 and VEGFR-1 receptors. In thepresent study, we show that the Bmx gene is expressed in endothelialcells of certain blood vessels, in the atria of the heart, andin thymic and lingual epithelial cells. In the venous endothelium,only a weak Bmx signal was seen in the superior and inferior venaecavae near theheart.

Bmx expression was strong at sites where the blood pressure and blood flow are regulated in the more peripheral vessels andmore centrally, where atherosclerosis occurs, such as in the coronaryarteries, aorta, and carotid and cerebral arteries. Accordingto these data, the Bmx promoter could also be a potential toolfor studying the function of the arterial endothelium in transgenicmodels. By using the Bmx promoter, it could be possible to expressa gene of interest specifically in arterial endothelialcells.

Previously, ephrin B2, a transmembrane ligand, has been shown to be expressed in the arterial endothelium, but not in thevenous endothelium, in the earliest stages of vasculogenesis.Ephrin B2-knockout mice die in utero before E11.5 because of defectiveangiogenesis (1, 39). Recently, another membrane-bound signaltransduction molecule, Dll4, a member of the Delta family of Notchligands, was found to be expressed specifically in the arterialendothelium (33), and indeed Notch signaling was shown to berequired for vascular remodeling in mice (20).

During mouse development, primitive blood vessels begin to form at E8.0, and remodeling of capillaries into arteries is evidentin the yolk sac between E9.0 and E9.5 (39). Unlike ephrin B2or Dll4, Bmx was activated between E10.5 and 12.5, which suggeststhat Bmx does not participate in the initial stages of vasculogenesisor arteriogenesis of mouse embryos. The role of Bmx in endothelialcells, as well as the mechanisms that activate the Bmx promoterin arteries but not in veins, is unknown. However, our data showthat the Bmx TK activity is increased by VEGFR-1 and Tie-2 inendothelial cells and suggest a role for Bmx in the endothelialsignal transduction. Although embryos homozygous for a Tie-2-nullallele die at E9.5 (3, 30) and those lacking VEGFR-1 dieat E8.5 (6), our present study shows that the Bmx-null miceare viable and without an obvious phenotype, at least in the presentDBA/2 background. This suggests that Bmx signaling is a redundantpathway downstream of the Tie-2 receptor. In the case of VEGFR-1,such deductions are less obvious as the TK domain of this receptoralso can be deleted without an obvious resulting phenotype (10).The Bmx protein has previously been shown to regulate granulocyticdifferentiation of cultured myeloid progenitor cells (4). However,in differential counting of peripheral blood leukocytes, no significantdifferences could be detected between wt and knockout mice. Theseresults further point to the redundancy of the functions of theBmxTK.

Interestingly, both the Tie-2 and the Bmx TKs are involved in endothelial cell adhesion and migration and the activation ofthe Stat transcription factors (16, 19, 29, 34; our unpublisheddata). Thus, it is possible that Bmx provides the Tie-2 receptora signal amplifier and a link to the cytoskeleton and cell adhesion,which allows the Tie-2 receptor, which is constitutively expressedin the various endothelia, to induce a tightly adherent endothelialcell phenotype in arteriae, where high blood flow and shear stressforces operate. In this way, Bmx function could be involved incellular responses to the stress caused by blood flow and pressureor perhaps in interactions of endothelial cells with the muscularwalls of thearteries.

We have previously shown that Bmx is regulated via phosphatidylinositol 3-kinase (4). This provides a possible route foractivation of Bmx by Tie-2 receptor, as it also has been shownpreviously that p85 becomes highly phosphorylated when coexpressedwith activated Tie-2 and following Ang-1 stimulation (11, 17).However, other possibilities also exist. For example, the activationsignal could be mediated by some of the docking proteins bindingto the Tie-2 receptors (see reference 26). We are currentlyinvestigating these proteins in order to exactly determine theroute of Bmxactivation.

	ACKNOWLEDGMENTS

I. Rajantie and N. Ekman contributed equally to thiswork.

We are grateful to Masabumi Shibuya and Lena Claesson-Welsh for kindly providing the Abs specified in Materials and Methods.We also thank the laboratory technicians Tapio Tainola, PipsaYlikantola, Eija Koivunen, and Riikka Kivirikko for excellenttechnicalassistance.

This work was supported by the Finnish Cancer Organizations, the Finnish Academy, the Sigrid Juselius Foundation, the Universityof Helsinki, and the European Union BioTechnology program (BIO4-CT98-0142).In addition, N.E. was supported by grants from the Helsinki UniversityBiomedical Graduate School, from the Research and Science Foundationof Farmos, and from the Finnish Foundation for CardiovascularResearch.

	FOOTNOTES

^* Corresponding author. Mailing address: Molecular/Cancer Biology Laboratory, Biomedicum Helsinki, P.O. Box 63 (Haartmaninkatu8), 00014 University of Helsinki, Finland. Phone: 358-9-1912 5511.Fax: 358-9-1912 5510. E-mail: Kari.Alitalo{at}Helsinki.FI.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Adams, R. H., G. A. Wilkinson, C. Weiss, F. Diella, N. W. Gale, U. Deutsch, W. Risau, and R. Klein. 1999. Roles of ephrinB ligands and EphB receptors in cardiovascular development: demarcation of arterial/venous domains, vascular morphogenesis, and sprouting angiogenesis. Genes Dev. 13:295-306[Abstract/Free Full Text].

2. Carmeliet, P., L. Kieckens, L. Schoonjans, B. Ream, A. van Nuffelen, G. Prendergast, M. Cole, R. Bronson, D. Collen, and R. C. Mulligan. 1993. Plasminogen activator inhibitor-1 gene-deficient mice. I. Generation by homologous recombination and characterization. J. Clin. Investig. 92:2746-2755.

3. Dumont, D. J., G. Gradwohl, G. H. Fong, M. C. Puri, M. Gertsenstein, A. Auerbach, and M. L. Breitman. 1994. Dominant-negative and targeted null mutations in the endothelial receptor tyrosine kinase, tek, reveal a critical role in vasculogenesis of the embryo. Genes Dev. 8:1897-1909[Abstract/Free Full Text].

4. Ekman, N., E. Arighi, I. Rajantie, P. Saharinen, A. Ristimäki, O. Silvennoinen, and K. Alitalo. 2000. The Bmx tyrosine kinase is activated by IL-3 and G-CSF in a PI-3K dependent manner. Oncogene 19:4151-4158[CrossRef][Medline].

5. Ekman, N., A. Lymboussaki, I. Västrik, K. Sarvas, A. Kaipainen, and K. Alitalo. 1997. The Bmx tyrosine kinase is specifically expressed in the endocardium and the endothelium of large arteries. Circulation 96:1729-1732[Abstract/Free Full Text].

6. Fong, G. H., J. Rossant, M. Gertsenstein, and M. L. Breitman. 1995. Role of the Flt-1 receptor tyrosine kinase in regulating the assembly of vascular endothelium. Nature 376:66-70[CrossRef][Medline].

7. Freshney, R. I. 1998. Culture of animal cells. A manual of basic techniques, 2nd ed. Alan R. Liss, New York, N.Y.

8. Gale, N. W., and G. D. Yancopoulos. 1999. Growth factors acting via endothelial cell-specific receptor tyrosine kinases: VEGFs, angiopoietins, and ephrins in vascular development. Genes Dev. 13:1055-1066[Free Full Text].

9. Giancotti, F. G., and E. Ruoslahti. 1999. Integrin signaling. Science 285:1028-1032[Abstract/Free Full Text].

10. Hiratsuka, S., O. Minowa, J. Kuno, T. Noda, and M. Shibuya. 1998. Flt-1 lacking the tyrosine kinase domain is sufficient for normal development and angiogenesis in mice. Proc. Natl. Acad. Sci. USA 95:9349-9354[Abstract/Free Full Text].

11. Jones, N., Z. Master, J. Jones, D. Bouchard, Y. Gunji, H. Sasaki, R. Daly, K. Alitalo, and D. J. Dumont. 1999. Identification of Tek/Tie2 binding partners. Binding to a multifunctional docking site mediates cell survival and migration. J. Biol. Chem. 274:30896-30905[Abstract/Free Full Text].

12. Jussila, L., R. Valtola, T. A. Partanen, P. Salven, P. Heikkila, M. T. Matikainen, R. Renkonen, A. Kaipainen, M. Detmar, E. Tschachler, R. Alitalo, and K. Alitalo. 1998. Lymphatic endothelium and Kaposi's sarcoma spindle cells detected by antibodies against the vascular endothelial growth factor receptor-3. Cancer Res. 58:1599-1604[Abstract/Free Full Text].

13. Kallioniemi, O. P., A. Kallioniemi, L. Mascio, D. Sudar, D. Pinkel, L. Deaven, and J. Gray. 1994. Physical mapping of chromosome 17 cosmids by fluorescence in situ hybridization and digital image analysis. Genomics 20:125-128[CrossRef][Medline].

14. Karkkainen, M. J., and T. V. Petrova. 2000. Vascular endothelial growth factor receptors in the regulation of angiogenesis and lymphangiogenesis. Oncogene 19:5598-5605[CrossRef][Medline].

15. Kaukonen, J., I. Lahtinen, S. Laine, K. Alitalo, and A. Palotie. 1996. Bmx tyrosine kinase gene is expressed in granulocytes and myeloid leukemias. Br. J. Haematol. 94:455-460[Medline].

16. Kim, I., H. G. Kim, S. O. Moon, S. W. Chae, J. N. So, K. N. Koh, B. C. Ahn, and G. Y. Koh. 2000. Angiopoietin-1 induces endothelial cell sprouting through the activation of focal adhesion kinase and plasmin secretion. Circ. Res. 86:952-959[Abstract/Free Full Text].

17. Kontos, C. D., T. P. Stauffer, W. P. Yang, J. D. York, L. Huang, M. A. Blanar, T. Meyer, and K. G. Peters. 1998. Tyrosine 1101 of Tie2 is the major site of association of p85 and is required for activation of phosphatidylinositol 3-kinase and Akt. Mol. Cell. Biol. 18:4131-4140[Abstract/Free Full Text].

18. Korhonen, J., I. Lahtinen, M. Halmekyto, L. Alhonen, J. Janne, D. Dumont, and K. Alitalo. 1995. Endothelial-specific gene expression directed by the tie gene promoter in vivo. Blood 86:1828-1835[Abstract/Free Full Text].

19. Korpelainen, E. I., M. Karkkainen, Y. Gunji, M. Vikkula, and K. Alitalo. 1999. Endothelial receptor tyrosine kinases activate the STAT signaling pathway: mutant Tie-2 causing venous malformations signals a distinct STAT activation response. Oncogene 18:1-8[CrossRef][Medline].

20. Krebs, L. T., Y. Xue, C. R. Norton, J. R. Shutter, M. Maguire, J. P. Sundberg, D. Gallahan, V. Closson, J. Kitajewski, R. Callahan, G. H. Smith, K. L. Stark, and T. Gridley. 2000. Notch signaling is essential for vascular morphogenesis in mice. Genes Dev. 14:1343-1352[Abstract/Free Full Text].

21. Kukk, E., U. Wartiovaara, Y. Gunji, J. Kaukonen, H. J. Buhring, I. Rappold, M. T. Matikainen, P. Vihko, J. Partanen, A. Palotie, K. Alitalo, and R. Alitalo. 1997. Analysis of Tie receptor tyrosine kinase in haemopoietic progenitor and leukaemia cells. Br. J. Haematol. 98:195-203[CrossRef][Medline].

22. Luscher, T. F., and F. C. Tanner. 1993. Endothelial regulation of vascular tone and growth. Am. J. Hypertens. 6:283S-293S[Medline].

23. Lusis, A. J. 2000. Atherosclerosis. Nature 407:233-241[CrossRef][Medline].

24. Mano, H. 1999. Tec family of protein-tyrosine kinases: an overview of their structure and function. Cytokine Growth Factor Rev. 10:267-280[CrossRef][Medline].

25. Partanen, J., E. Armstrong, T. P. Makela, J. Korhonen, M. Sandberg, R. Renkonen, S. Knuutila, K. Huebner, and K. Alitalo. 1992. A novel endothelial cell surface receptor tyrosine kinase with extracellular epidermal growth factor homology domains. Mol. Cell. Biol. 12:1698-1707[Abstract/Free Full Text].

26. Partanen, J., and D. J. Dumont. 1999. Functions of Tie1 and Tie2 receptor tyrosine kinases in vascular development. Curr. Top. Microbiol. Immunol. 273:159-172.

27. Pawson, T., and P. Nash. 2000. Protein-protein interactions define specificity in signal transduction. Genes Dev. 14:1027-1047[Free Full Text].

28. Risau, W. 1995. Differentiation of endothelium. FASEB J. 9:926-933[Abstract].

29. Saharinen, P., N. Ekman, K. Sarvas, P. Parker, K. Alitalo, and O. Silvennoinen. 1997. The Bmx tyrosine kinase induces activation of the Stat signalling pathway, which is specifically inhibited by PKC $delta$ . Blood 90:4341-4353[Abstract/Free Full Text].

30. Sato, T. N., Y. Tozawa, U. Deutsch, K. Wolburg-Buchholz, Y. Fujiwara, M. Gendron-Maguire, T. Gridley, H. Wolburg, W. Risau, and Y. Qin. 1995. Distinct roles of the receptor tyrosine kinases Tie-1 and Tie-2 in blood vessel formation. Nature 376:70-74[CrossRef][Medline].

31. Schlessinger, J. 2000. Cell signaling by receptor tyrosine kinases. Cell 103:211-225[CrossRef][Medline].

32. Shalaby, F., J. Rossant, T. P. Yamaguchi, M. Gertsenstein, X. F. Wu, M. L. Breitman, and A. C. Schuh. 1995. Failure of blood-island formation and vasculogenesis in Flk-1-deficient mice. Nature 376:62-66[CrossRef][Medline].

33. Shutter, J. R., S. Scully, W. Fan, W. G. Richards, J. Kitajewski, G. A. Deblandre, C. R. Kintner, and K. L. Stark. 2000. Dll4, a novel Notch ligand expressed in arterial endothelium. Genes Dev. 14:1313-1318[Abstract/Free Full Text].

34. Takakura, N., X. L. Huang, T. Naruse, I. Hamaguchi, D. J. Dumont, G. D. Yancopoulos, and T. Suda. 1998. Critical role of the TIE2 endothelial cell receptor in the development of definitive hematopoiesis. Immunity 9:677-686[CrossRef][Medline].

35. Tamagnone, L., I. Lahtinen, T. Mustonen, K. Virtaneva, F. Francis, F. Muscatelli, R. Alitalo, C. I. Smith, C. Larsson, and K. Alitalo. 1994. BMX, a novel nonreceptor tyrosine kinase gene of the BTK/ITK/TEC/TXK family located in chromosome Xp22.2. Oncogene 9:3683-3688[Medline].

36. Thurston, G., T. J. Murphy, P. Baluk, J. R. Lindsey, and D. M. McDonald. 1998. Angiogenesis in mice with chronic airway inflammation: strain-dependent differences. Am. J. Pathol. 153:1099-1112[Abstract/Free Full Text].

37. Vikkula, M., L. M. Boon, K. L. Carraway, 3rd, J. T. Calvert, A. J. Diamonti, B. Goumnerov, K. A. Pasyk, D. A. Marchuk, M. L. Warman, L. C. Cantley, J. B. Mulliken, and B. R. Olsen. 1996. Vascular dysmorphogenesis caused by an activating mutation in the receptor tyrosine kinase TIE2. Cell 87:1181-1190[CrossRef][Medline].

38. Vuori, K. 1998. Integrin signaling: tyrosine phosphorylation events in focal adhesions. J. Membr. Biol. 165:191-199[CrossRef][Medline].

39. Wang, H. U., Z. F. Chen, and D. J. Anderson. 1998. Molecular distinction and angiogenic interaction between embryonic arteries and veins revealed by ephrin-B2 and its receptor Eph-B4. Cell 93:741-753[CrossRef][Medline].

40. Weil, D., M. A. Power, S. I. Smith, and C. H. Li. 1998. Predominant expression of murine Bmx tyrosine kinase in the granulo-monocytic lineage. Blood 90:4332-4340[Abstract/Free Full Text].

41. Yang, W. C., Y. Collette, Y. Nunes, and D. Olive. 2000. Tec kinases: a family with multiple roles in immunity. Immunity 12:373-382[CrossRef][Medline].

This article has been cited by other articles:

Mitchell-Jordan, S. A., Holopainen, T., Ren, S., Wang, S., Warburton, S., Zhang, M. J., Alitalo, K., Wang, Y., Vondriska, T. M. (2008). Loss of Bmx Nonreceptor Tyrosine Kinase Prevents Pressure Overload-Induced Cardiac Hypertrophy. Circ. Res. 103: 1359-1362 [Abstract] [Full Text]
Melcher, M., Unger, B., Schmidt, U., Rajantie, I. A., Alitalo, K., Ellmeier, W. (2008). Essential Roles for the Tec Family Kinases Tec and Btk in M-CSF Receptor Signaling Pathways That Regulate Macrophage Survival. J. Immunol. 180: 8048-8056 [Abstract] [Full Text]
Tu, T., Thotala, D., Geng, L., Hallahan, D. E., Willey, C. D. (2008). Bone Marrow X Kinase-Mediated Signal Transduction in Irradiated Vascular Endothelium. Cancer Res. 68: 2861-2869 [Abstract] [Full Text]
Jiang, X., Borgesi, R. A., McKnight, N. C., Kaur, R., Carpenter, C. L., Balk, S. P. (2007). Activation of Nonreceptor Tyrosine Kinase Bmx/Etk Mediated by Phosphoinositide 3-Kinase, Epidermal Growth Factor Receptor, and ErbB3 in Prostate Cancer Cells. J. Biol. Chem. 282: 32689-32698 [Abstract] [Full Text]
Dai, B., Kim, O., Xie, Y., Guo, Z., Xu, K., Wang, B., Kong, X., Melamed, J., Chen, H., Bieberich, C. J., Borowsky, A. D., Kung, H.-J., Wei, G., Ostrowski, M. C., Brodie, A., Qiu, Y. (2006). Tyrosine Kinase Etk/BMX Is Up-regulated in Human Prostate Cancer and Its Overexpression Induces Prostate Intraepithelial Neoplasia in Mouse. Cancer Res. 66: 8058-8064 [Abstract] [Full Text]
Mathur, P., Kaga, S., Zhan, L., Das, D. K., Maulik, N. (2005). Potential candidates for ischemic preconditioning-associated vascular growth pathways revealed by antibody array. Am. J. Physiol. Heart Circ. Physiol. 288: H3006-H3010 [Abstract] [Full Text]
Paavonen, K., Ekman, N., Wirzenius, M., Rajantie, I., Poutanen, M., Alitalo, K. (2004). Bmx Tyrosine Kinase Transgene Induces Skin Hyperplasia, Inflammatory Angiogenesis, and Accelerated Wound Healing. Mol. Biol. Cell 15: 4226-4233 [Abstract] [Full Text]
Shiu, S.-H., Li, W.-H. (2004). Origins, Lineage-Specific Expansions, and Multiple Losses of Tyrosine Kinases in Eukaryotes. Mol Biol Evol 21: 828-840 [Abstract] [Full Text]
Zhang, R., Xu, Y., Ekman, N., Wu, Z., Wu, J., Alitalo, K., Min, W. (2003). Etk/Bmx Transactivates Vascular Endothelial Growth Factor 2 and Recruits Phosphatidylinositol 3-Kinase to Mediate the Tumor Necrosis Factor-induced Angiogenic Pathway. J. Biol. Chem. 278: 51267-51276 [Abstract] [Full Text]
Hamada, K., Oike, Y., Ito, Y., Maekawa, H., Miyata, K., Shimomura, T., Suda, T. (2003). Distinct Roles of Ephrin-B2 Forward and EphB4 Reverse Signaling in Endothelial Cells. Arterioscler. Thromb. Vasc. Bio. 23: 190-197 [Abstract] [Full Text]
Pan, S., An, P., Zhang, R., He, X., Yin, G., Min, W. (2002). Etk/Bmx as a Tumor Necrosis Factor Receptor Type 2-Specific Kinase: Role in Endothelial Cell Migration and Angiogenesis. Mol. Cell. Biol. 22: 7512-7523 [Abstract] [Full Text]
Vargas, L., Nore, B. F., Berglof, A., Heinonen, J. E., Mattsson, P. T., Smith, C. I. E., Mohamed, A. J. (2002). Functional Interaction of Caveolin-1 with Bruton's Tyrosine Kinase and Bmx. J. Biol. Chem. 277: 9351-9357 [Abstract] [Full Text]
Takesono, A., Finkelstein, L. D., Schwartzberg, P. L. (2002). Beyond calcium: new signaling pathways for Tec family kinases. J. Cell Sci. 115: 3039-3048 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Rajantie, I.
	Articles by Alitalo, K.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Rajantie, I.
	Articles by Alitalo, K.

1.	Adams, R. H., G. A. Wilkinson, C. Weiss, F. Diella, N. W. Gale, U. Deutsch, W. Risau, and R. Klein. 1999. Roles of ephrinB ligands and EphB receptors in cardiovascular development: demarcation of arterial/venous domains, vascular morphogenesis, and sprouting angiogenesis. Genes Dev. 13:295-306[Abstract/Free Full Text].
2.	Carmeliet, P., L. Kieckens, L. Schoonjans, B. Ream, A. van Nuffelen, G. Prendergast, M. Cole, R. Bronson, D. Collen, and R. C. Mulligan. 1993. Plasminogen activator inhibitor-1 gene-deficient mice. I. Generation by homologous recombination and characterization. J. Clin. Investig. 92:2746-2755.
3.	Dumont, D. J., G. Gradwohl, G. H. Fong, M. C. Puri, M. Gertsenstein, A. Auerbach, and M. L. Breitman. 1994. Dominant-negative and targeted null mutations in the endothelial receptor tyrosine kinase, tek, reveal a critical role in vasculogenesis of the embryo. Genes Dev. 8:1897-1909[Abstract/Free Full Text].
4.	Ekman, N., E. Arighi, I. Rajantie, P. Saharinen, A. Ristimäki, O. Silvennoinen, and K. Alitalo. 2000. The Bmx tyrosine kinase is activated by IL-3 and G-CSF in a PI-3K dependent manner. Oncogene 19:4151-4158[CrossRef][Medline].
5.	Ekman, N., A. Lymboussaki, I. Västrik, K. Sarvas, A. Kaipainen, and K. Alitalo. 1997. The Bmx tyrosine kinase is specifically expressed in the endocardium and the endothelium of large arteries. Circulation 96:1729-1732[Abstract/Free Full Text].
6.	Fong, G. H., J. Rossant, M. Gertsenstein, and M. L. Breitman. 1995. Role of the Flt-1 receptor tyrosine kinase in regulating the assembly of vascular endothelium. Nature 376:66-70[CrossRef][Medline].
7.	Freshney, R. I. 1998. Culture of animal cells. A manual of basic techniques, 2nd ed. Alan R. Liss, New York, N.Y.
8.	Gale, N. W., and G. D. Yancopoulos. 1999. Growth factors acting via endothelial cell-specific receptor tyrosine kinases: VEGFs, angiopoietins, and ephrins in vascular development. Genes Dev. 13:1055-1066[Free Full Text].
9.	Giancotti, F. G., and E. Ruoslahti. 1999. Integrin signaling. Science 285:1028-1032[Abstract/Free Full Text].
10.	Hiratsuka, S., O. Minowa, J. Kuno, T. Noda, and M. Shibuya. 1998. Flt-1 lacking the tyrosine kinase domain is sufficient for normal development and angiogenesis in mice. Proc. Natl. Acad. Sci. USA 95:9349-9354[Abstract/Free Full Text].
11.	Jones, N., Z. Master, J. Jones, D. Bouchard, Y. Gunji, H. Sasaki, R. Daly, K. Alitalo, and D. J. Dumont. 1999. Identification of Tek/Tie2 binding partners. Binding to a multifunctional docking site mediates cell survival and migration. J. Biol. Chem. 274:30896-30905[Abstract/Free Full Text].
12.	Jussila, L., R. Valtola, T. A. Partanen, P. Salven, P. Heikkila, M. T. Matikainen, R. Renkonen, A. Kaipainen, M. Detmar, E. Tschachler, R. Alitalo, and K. Alitalo. 1998. Lymphatic endothelium and Kaposi's sarcoma spindle cells detected by antibodies against the vascular endothelial growth factor receptor-3. Cancer Res. 58:1599-1604[Abstract/Free Full Text].
13.	Kallioniemi, O. P., A. Kallioniemi, L. Mascio, D. Sudar, D. Pinkel, L. Deaven, and J. Gray. 1994. Physical mapping of chromosome 17 cosmids by fluorescence in situ hybridization and digital image analysis. Genomics 20:125-128[CrossRef][Medline].
14.	Karkkainen, M. J., and T. V. Petrova. 2000. Vascular endothelial growth factor receptors in the regulation of angiogenesis and lymphangiogenesis. Oncogene 19:5598-5605[CrossRef][Medline].
15.	Kaukonen, J., I. Lahtinen, S. Laine, K. Alitalo, and A. Palotie. 1996. Bmx tyrosine kinase gene is expressed in granulocytes and myeloid leukemias. Br. J. Haematol. 94:455-460[Medline].
16.	Kim, I., H. G. Kim, S. O. Moon, S. W. Chae, J. N. So, K. N. Koh, B. C. Ahn, and G. Y. Koh. 2000. Angiopoietin-1 induces endothelial cell sprouting through the activation of focal adhesion kinase and plasmin secretion. Circ. Res. 86:952-959[Abstract/Free Full Text].
17.	Kontos, C. D., T. P. Stauffer, W. P. Yang, J. D. York, L. Huang, M. A. Blanar, T. Meyer, and K. G. Peters. 1998. Tyrosine 1101 of Tie2 is the major site of association of p85 and is required for activation of phosphatidylinositol 3-kinase and Akt. Mol. Cell. Biol. 18:4131-4140[Abstract/Free Full Text].
18.	Korhonen, J., I. Lahtinen, M. Halmekyto, L. Alhonen, J. Janne, D. Dumont, and K. Alitalo. 1995. Endothelial-specific gene expression directed by the tie gene promoter in vivo. Blood 86:1828-1835[Abstract/Free Full Text].
19.	Korpelainen, E. I., M. Karkkainen, Y. Gunji, M. Vikkula, and K. Alitalo. 1999. Endothelial receptor tyrosine kinases activate the STAT signaling pathway: mutant Tie-2 causing venous malformations signals a distinct STAT activation response. Oncogene 18:1-8[CrossRef][Medline].
20.	Krebs, L. T., Y. Xue, C. R. Norton, J. R. Shutter, M. Maguire, J. P. Sundberg, D. Gallahan, V. Closson, J. Kitajewski, R. Callahan, G. H. Smith, K. L. Stark, and T. Gridley. 2000. Notch signaling is essential for vascular morphogenesis in mice. Genes Dev. 14:1343-1352[Abstract/Free Full Text].
21.	Kukk, E., U. Wartiovaara, Y. Gunji, J. Kaukonen, H. J. Buhring, I. Rappold, M. T. Matikainen, P. Vihko, J. Partanen, A. Palotie, K. Alitalo, and R. Alitalo. 1997. Analysis of Tie receptor tyrosine kinase in haemopoietic progenitor and leukaemia cells. Br. J. Haematol. 98:195-203[CrossRef][Medline].
22.	Luscher, T. F., and F. C. Tanner. 1993. Endothelial regulation of vascular tone and growth. Am. J. Hypertens. 6:283S-293S[Medline].
23.	Lusis, A. J. 2000. Atherosclerosis. Nature 407:233-241[CrossRef][Medline].
24.	Mano, H. 1999. Tec family of protein-tyrosine kinases: an overview of their structure and function. Cytokine Growth Factor Rev. 10:267-280[CrossRef][Medline].
25.	Partanen, J., E. Armstrong, T. P. Makela, J. Korhonen, M. Sandberg, R. Renkonen, S. Knuutila, K. Huebner, and K. Alitalo. 1992. A novel endothelial cell surface receptor tyrosine kinase with extracellular epidermal growth factor homology domains. Mol. Cell. Biol. 12:1698-1707[Abstract/Free Full Text].
26.	Partanen, J., and D. J. Dumont. 1999. Functions of Tie1 and Tie2 receptor tyrosine kinases in vascular development. Curr. Top. Microbiol. Immunol. 273:159-172.
27.	Pawson, T., and P. Nash. 2000. Protein-protein interactions define specificity in signal transduction. Genes Dev. 14:1027-1047[Free Full Text].
28.	Risau, W. 1995. Differentiation of endothelium. FASEB J. 9:926-933[Abstract].
29.	Saharinen, P., N. Ekman, K. Sarvas, P. Parker, K. Alitalo, and O. Silvennoinen. 1997. The Bmx tyrosine kinase induces activation of the Stat signalling pathway, which is specifically inhibited by PKC $delta$ . Blood 90:4341-4353[Abstract/Free Full Text].
30.	Sato, T. N., Y. Tozawa, U. Deutsch, K. Wolburg-Buchholz, Y. Fujiwara, M. Gendron-Maguire, T. Gridley, H. Wolburg, W. Risau, and Y. Qin. 1995. Distinct roles of the receptor tyrosine kinases Tie-1 and Tie-2 in blood vessel formation. Nature 376:70-74[CrossRef][Medline].
31.	Schlessinger, J. 2000. Cell signaling by receptor tyrosine kinases. Cell 103:211-225[CrossRef][Medline].
32.	Shalaby, F., J. Rossant, T. P. Yamaguchi, M. Gertsenstein, X. F. Wu, M. L. Breitman, and A. C. Schuh. 1995. Failure of blood-island formation and vasculogenesis in Flk-1-deficient mice. Nature 376:62-66[CrossRef][Medline].
33.	Shutter, J. R., S. Scully, W. Fan, W. G. Richards, J. Kitajewski, G. A. Deblandre, C. R. Kintner, and K. L. Stark. 2000. Dll4, a novel Notch ligand expressed in arterial endothelium. Genes Dev. 14:1313-1318[Abstract/Free Full Text].
34.	Takakura, N., X. L. Huang, T. Naruse, I. Hamaguchi, D. J. Dumont, G. D. Yancopoulos, and T. Suda. 1998. Critical role of the TIE2 endothelial cell receptor in the development of definitive hematopoiesis. Immunity 9:677-686[CrossRef][Medline].
35.	Tamagnone, L., I. Lahtinen, T. Mustonen, K. Virtaneva, F. Francis, F. Muscatelli, R. Alitalo, C. I. Smith, C. Larsson, and K. Alitalo. 1994. BMX, a novel nonreceptor tyrosine kinase gene of the BTK/ITK/TEC/TXK family located in chromosome Xp22.2. Oncogene 9:3683-3688[Medline].
36.	Thurston, G., T. J. Murphy, P. Baluk, J. R. Lindsey, and D. M. McDonald. 1998. Angiogenesis in mice with chronic airway inflammation: strain-dependent differences. Am. J. Pathol. 153:1099-1112[Abstract/Free Full Text].
37.	Vikkula, M., L. M. Boon, K. L. Carraway, 3rd, J. T. Calvert, A. J. Diamonti, B. Goumnerov, K. A. Pasyk, D. A. Marchuk, M. L. Warman, L. C. Cantley, J. B. Mulliken, and B. R. Olsen. 1996. Vascular dysmorphogenesis caused by an activating mutation in the receptor tyrosine kinase TIE2. Cell 87:1181-1190[CrossRef][Medline].
38.	Vuori, K. 1998. Integrin signaling: tyrosine phosphorylation events in focal adhesions. J. Membr. Biol. 165:191-199[CrossRef][Medline].
39.	Wang, H. U., Z. F. Chen, and D. J. Anderson. 1998. Molecular distinction and angiogenic interaction between embryonic arteries and veins revealed by ephrin-B2 and its receptor Eph-B4. Cell 93:741-753[CrossRef][Medline].
40.	Weil, D., M. A. Power, S. I. Smith, and C. H. Li. 1998. Predominant expression of murine Bmx tyrosine kinase in the granulo-monocytic lineage. Blood 90:4332-4340[Abstract/Free Full Text].
41.	Yang, W. C., Y. Collette, Y. Nunes, and D. Olive. 2000. Tec kinases: a family with multiple roles in immunity. Immunity 12:373-382[CrossRef][Medline].