Biostatistical study on the arrangement of the superficial veins of the cubital fossa in Iraqis

A study of the arrangement of the superficial veins of the cubital fossa was made on 300 students and staff of the Military Medical College and the AlMustansiriya College of Medicine. Six types of variations of arrangement of the veins were found, two of which have not been mentioned before. The commonest type was that the median vein of the forearm divides in the cubital fossa into 2 veins, one of which joins the basilic vein, and the other the cephalic vein, although in a few cases this joining (or arrangement), occurred above the cubital fossa. The arrangements which have not been mentioned before were that the communication between basilic and cephalic veins was through a horizontal venous connection between 1 of the tributaries of these 2 veins and the basilic vein, and that the median vein of the forearm divides into median cephalic and median basilic, and a vein from the front of the forearm drains into the median basilic vein.     

Action of ACTH in the luteal ovary.

Oestrous rats and golden hamsters were anesthetized with pentobarbital, one of the femoral arteries and veins and one of the ovarian veins were cannulated. Blood fractions were collected from the ovary. After the first two fractions synthetic adrenocorticotropic hormone (ACTH) or human chorionic gonadotropin (hCG) was injected i.v. Blood pressures and ovarian blood flow were continuously recorded. Progesterone (P) and oestradiol-17 beta (E2) were determined from the ovarian venous blood by radioimmunoassay (RIA). ACTH induced a temporary elevation in the ovarian blood flow, P and E2 secretion both in rats and hamsters. In rats and hamsters hCG induced a continuous elevation in P secretion but the ovarian blood flow and E2 secretion remained unchanged. Luteal cells from pseudopregnant rats or oestrous hamsters were dispersed with collagenase and incubated with ACTH or hCG. A sample of the cells was preincubated with polymixin-B, indomethacin or ibuprofen. P and 6-keto-prostaglandin F1 alpha (6-keto-PGF1 alpha) contents of the medium and cyclic 3,5 adenosine monophosphate (cAMP) content of the cells were determined by RIA. ACTH stimulated the release of 6-keto-PGF1 alpha and the secretion of P from the luteal cells of both species, which was inhibited by indomethacin or ibuprofen, but ACTH did not alter the cAMP content of luteal cells. The polymixin-B prevented ACTH to stimulate P secretion, but it did not elevate the 6-keto-PGF1 alpha release, while the cAMP content of the cells remained unchanged. It is supposed that the polyphosphoinositol-Ca(2+)-protein kinase-C second messenger system is involved in the ACTH induced stimulation of P secretion.     

Integrated Proteomic Analysis of Human Cancer Cells and Plasma from Tumor Bearing Mice for Ovarian Cancer Biomarker Discovery

Background

The complexity of the human plasma proteome represents a substantial challenge for biomarker discovery. Proteomic analysis of genetically engineered mouse models of cancer and isolated cancer cells and cell lines provide alternative methods for identification of potential cancer markers that would be detectable in human blood using sensitive assays. The goal of this work is to evaluate the utility of an integrative strategy using these two approaches for biomarker discovery.

Methodology/Principal Findings

We investigated a strategy that combined quantitative plasma proteomics of an ovarian cancer mouse model with analysis of proteins secreted or shed by human ovarian cancer cells. Of 106 plasma proteins identified with increased levels in tumor bearing mice, 58 were also secreted or shed from ovarian cancer cells. The remainder consisted primarily of host-response proteins. Of 25 proteins identified in the study that were assayed, 8 mostly secreted proteins common to mouse plasma and human cancer cells were significantly upregulated in a set of plasmas from ovarian cancer patients. Five of the eight proteins were confirmed to be upregulated in a second independent set of ovarian cancer plasmas, including in early stage disease.

Conclusions/Significance

Integrated proteomic analysis of cancer mouse models and human cancer cell populations provides an effective approach to identify potential circulating protein biomarkers.     

Local adjustment of blood and lymph circulation in the hormonal regulation of reproduction in female pigs--facts, conclusions and suggestions for future research

Arteries, veins, capillaries and lymphatic vessels situated in the mesovarium and mesosalpinx of domestic animal species (pig, cow, sheep) form the periovarian vascular complex. Particular components of the periovarian vascular complex interact functionally and morphologically creating a specific environment for numerous physiological processes. The complex plays an essential role in the system of the retrograde transfer of the ovarian hormones. This phenomenon is especially well documented in pigs. The efficiency of the retrograde transfer of estradiol and progesterone from blood and lymph leaving the gonad to blood of the ovarian artery (expressed as percentage of their concentration in the ovarian venous blood) as well as the rate of the retrograde transfer of these hormones to the ovary (measured in nanograms or picograms per minute) is presented and discussed in this paper. No simple relationship was found between hormone concentration in ovarian venous effluent and the efficiency or the rate of their retrograde transfer during the estrous cycle. It appears that two processes contribute to the highly efficient retrograde transfer of ovarian hormones into the ovary in the periovarian vascular complex: 1/ direct hormone permeation from the ovarian vein into the adjacent branches of the ovarian artery through the counter-current mechanism; 2/ indirect permeation of ovarian hormones consisting of two stages. The first stage includes the permeation of hormones from lymph leaving the ovary via the subovarian lymphatic vascular network as well as lymph and venous blood, leaving the mesosalpinx and going to capillaries and tiny venous vessels in the entire mesovarium. These tiny mesovarium vessels connect and then branch out again to form the veno-venous network on the surface of branches of the ovarian artery. The second stage includes the permeation of hormones from the veno-venous blood into the branches of the ovarian artery. The authors present a hypothesis that the retrograde transfer of ovarian hormones may participate in the feedback regulation of ovarian function. The relationship between the retrograde transfer of ovarian hormones in the area of periovarian vascular complex and local elevation of steroid hormone concentrations in blood supplying the oviduct and uterus is presented. The paper also includes suggestions for future research.     

The extrinsic blood vessels of the ovary of the sheep.

The extrinsic ovarian blood vessels were studied in 134 ewes. In view of recent evidence that uterine luteolysis may involve venoarterial transfer of prostaglandin F2alpha in the ovarian pedicle, particular attention was paid to the interrelationships between veins and arteries. The ovarian artery and utero-ovarian vein are large vessels of conventional structure and lie in close apposition. Their walls are slightly thinner on their apposing sides. The ovarian branches of the ovarian artery are very tortuous, and closely intertwined with the plexiform ovarian branches of the utero-ovarian vein. An extensive plexus of small veins surrounds the ovarian artery and its ovarian branches. Within this plexus are many thin-walled, dilated regions, interspersed with narrow, thick-walled segments. Valves are inconstantly present at sites of entry of branches of the plexus into the major veins. Small numbers of arterio-venous anastomoses are present in the distal part of the ovarian pedicle. Unless blood can flow in a veno-arterial direction through arterio-venous anastomoses or capillary beds, the structural barrier between uterine venous and ovarian arterial blood is substantial.     

To be or not to be: postcubital vein in insects revealed by microtomography

To better understand insect evolution, fossils – mainly known by their wings – must be used as terminals in phylogenetic analyses. Such analyses are, however, rarely performed because of a lack of consensus on the homology of venation in insects. Researchers do not agree with the current concept on the exact number and identity of the main veins. Here, we confirm the presence, which has been in question since the early 20th century, of an independent main postcubital vein (PCu vein) between the cubital and anal veins (29 fossil and extant examined orders; > 85% of observed insects). The PCu vein corresponds to the so-called vein 1A or first anal vein. It is easily identified by the unique shape of its bulla. It may have several branches and be partially fused with the cubital and anal veins. Once the PCu vein was identified, we reconsidered as an example the particular case of the Phasmatodea, showing that extant stick insects have a unique venation among insects, with a reduced median vein and a simple cubital vein adjacent or fused to the PCu vein. This study is a new approach towards resolving wing vein homology issues, crucial for future large-scale phylogenetic analyses in insects combining extant and extinct taxa.     

上皮性卵巢肿瘤组织MKP-1及p-ERK1/2蛋白表达的研究

研究丝裂原活化蛋白激酶（mitogen activated protein kinase, MAPK） 相关蛋白丝裂原活化蛋白激酶磷酸酶（mitogen activated protein kinase phosphatase-1, MKP-1）和磷酸化细胞外信号调节激酶（phosphorylation extracellular signal-regulated kinases, p-ERK1/2）曲在上皮性卵巢肿瘤组织及正常卵巢组织中的表达差异,并探讨其在卵巢癌发生、发展中的作用,为卵巢癌的治疗提供新的思路及实验依据。选取64例上皮性卵巢癌、35例卵巢上皮性交界瘤及32例卵巢上皮性良性肿瘤患者的组织,另选取26例正常卵巢组织作对照,进行MKP-1及p-ERK1/2的免疫组化分析,并同时对其中部分病例进行上述蛋白的Western—blot研究。结果显示正常卵巢、良性肿瘤、交界瘤及卵巢癌组织MKP—1的表达依次递减,各组之间进行两两比较均有显著性差异（P〈0．01）,FIGOⅢ期与Ⅳ期卵巢癌组织MKP-1的表达显著低于Ⅰ期与Ⅱ期卵巢癌组织（P〈0．01）;而p-ERK1/2在正常卵巢、良性肿瘤、交界瘤及卵巢癌组织的表达依次递增．各组之间进行两两比较也均有显著性差异（P〈0．01）。FIGOⅢ期与Ⅳ期卵巢癌组织P～ERK1/2的表达显著高于Ⅰ期与Ⅱ期卵巢癌组织（P〈0．01）。且免疫组化及western—blot均显示MKP-1与p—ERK1/2在卵巢癌组织中的表达存在显著的负相关性,（r=-0．90,P〈0．01及r=-0．78,P〈0．01）。本研究结果表明MKP-1与p—ERK1/2的异常表达可能跟上皮性卵巢肿瘤的发生、发展有关,它们之间的表达失衡可能是卵巢癌发生、发展的原因之一．     

Observations on the vasculature of the reproductive tract in some Australian marsupials

The origin, distribution and structure of the blood vessels of the female reproductive tract and the testis of the brush possum (Trichosurus vulpecula) were studied using latex and silicone rubber casting and histological techniques. Latex casts of the vessels of the female tract were also studied in five macropod species – Macropus giganteus, M. eugenii, M. agilis, Megaleia rufa and Thylogale billardierii, and in the common wombat (Vombatus ursinus). The female reproductive tract in the brush possum was supplied and drained by four major sets of paired vessels – ovarian, cranial urogenital, caudal urogenital, and internal pudendal arteries and veins. These vessels formed substantial anastomoses with one another on each side of the midline, and also across-the-midline anastomoses. The proximal part of the ovarian artery ran in close apposition to the ovarian vein, which received one or more large uterine branches. In its distal protion the ovarian artery gave rise to a leash of small, tortuous ovarian branches, which wound around and between the plexiform ovarian veins. The testicular arteries and veins in this species also ran in close apposition to one another. Both arteries and veins branched into many smaller, mildly tortuous, parallel vessels in the spermatic cord, which reunited before entering the testis. The blood vessels of the reproductive tract in all of the macropod species studied, and in the common wombat, were basically similar to those of the brush possum. The intimate structural relationships between ovarian arteries and veins, and their ovarian branches, in these marsupials are suggestive of specializations for counter-current exchange between venous and arterial blood. However, in contrast to those of the testicular vessels where heat exchange is a demonstrated function, their physiological significance remains unknown.     

Plasma fibrinogen in female patients with genital cancer and its early stage

Changes of plasma fibrinogen derivates in 54 female patients suffering from carcinomas of the genital system (36 with cervix carcinoma, 9 with ovarian carcinomas, 7 with carcinomas of the corpus uteri, 1 woman with a vulva and 1 patient with vaginal carcinoma) and 6 females with cervical intraepithelial neoplasia were investigated. It was shown, that the fibrinogen content and the concentration of soluble fibrin monomer complexes in blood plasma depend on the extension of the clinically diagnosed tumor. Furthermore, differently degraded fibrinogens were demonstrated to exist in the blood circulation. The extent of fibrinogenolysis did not correlate with the clinically diagnosed tumor stage.     

FLIP、FADD在上皮性卵巢癌中表达及其临床意义

目的：研究FLIP、FADD在上皮性卵巢癌组织中的表达情况,探讨二者在上皮性卵巢癌发生发展中的作用及其临床意义。方法：采用免疫组化SP法及RT—PCR法检测44例上皮性卵巢癌及17例正常卵巢组织中FLIP、FADD的表达,并检测上皮性卵巢癌中PCNA的表达,分析FLIP,FADD表达与上皮性卵巢癌临床病理参数及PCNA表达的关系。结果：FLIP、FADD在上皮性卵巢癌组织中的阳性表达率,与正常卵巢组织相比,差异有统计学意义（P〈0．05）。FLIP,FADD表达与上皮性卵巢癌病理分级及临床分期有关,FLIP、FADD在I—II期中的阳性表达率,与III．IV期相比,差异有统计学意义（P〈0．05）。FLIP、FADD在病理组织学-1级中的阳性表达率,与2—3级相比,差异有统计学意义（P〈0．05）。FLIP、FADD的表达与患者年龄、组织学分型及淋巴结转移无关。上皮性卵巢癌组织中FLIP表达与PCNA表达成线性正相关,r分别0．880和0．564;FADD表达与PCNA表达成线性负相关,r分别为-0．591和-0．683。结论：FLIP、FADD与上皮性卵巢癌的发生发展密切相关,可能是治疗上皮性卵巢癌的潜在靶点。     

Characterization of a monoclonal antibody, OVB1, which binds to a unique determinant in human ovarian carcinomas and myeloid cells

A monoclonal antibody, OVB1, was generated against a human ovarian carcinoma cell line, OVCAR-3. The antigen reacting with this antibody was strongly expressed on the external surface of the plasma membrane of OVCAR-3 cells and cells of 4/4 other ovarian carcinoma lines. Variable density and homogeneity of expression was found on cells from 5/5 breast carcinoma lines. Various ovarian tumor specimens and normal human tissues were frozen, cryostat-sectioned, and examined for OVB1 reactivity using immunoperoxidase methods. A strong, uniform, homogeneous reaction on 10/10 ovarian carcinoma specimens and variable, non-homogeneous reactions on breast tumors were seen. Normal tissues reacting with the antibody include thyroid, pituitary pars intermedia, breast ductal epithelium, Auerbach's plexus and neuronal processes in the GI tract, colonic mucosal epithelium, and salivary gland ductal epithelium. Polymorphonuclear leukocytes, eosinophils, and approximately 13% of peripheral lymphocytes, as well as cells around germinal centers in lymph nodes and spleen, showed strong reactivity by immunofluorescence and/or immunoperoxidase. Expression of the OVB1 antigen in the myeloid cells of normal human bone marrow occurred from the promyelocyte stage through to more mature cells in a subpopulation of myeloblasts. Indirect immunofluorescence of live peripheral blood cells showed localization to the surface of PMNs, eosinophils, and certain lymphocytes. Double-immunofluorescence studies (with a direct fluorescein-anti-lactoferrin antibody conjugate) showed co-localization of OVB1 and OKM1 (anti-C3bi receptor) antibodies to specific granules of PMNs. Localization of OVB1 and OKM1 antibodies to granular structures in the PMN was confirmed by electron microscopy using the ferritin bridge technique. The antigen reacting with the OVB1 antibody was shown to be neuraminidase sensitive, but protease insensitive. The OVB1 monoclonal antibody may be useful in identification of ovarian tumors and subclassification of myeloid leukemias.     

Direct venous-arterial transfer of 125I-radiolabelled relaxin and tyrosine in the ovarian pedicle in sheep

125I-labelled relaxin and tyrosine were infused into the ovarian vein to investigate transfer to branches of the ovarian artery at the ovarian pedicle in sheep. The ovarian arteries supply the ovary, the oviduct, and the tip of the uterine horn. An exchange of relaxin (n = 24) and tyrosine (n = 18) was observed in blood samples collected from all branches of ovarian arteries. This is expressed as a ratio of radioactivity greater than 1 between jugular venous blood plasma and arterial blood plasma. The average ratio (+/- s.d.) over the total infusion period of 1 h was 1.42 (+/- 0.35) for relaxin and 1.69 (+/- 0.38) for tyrosine with maximal values up to 4.9 and 2.9, respectively. Of the total amount of substance infused (348 pmol/h), 0.22% of the relaxin and 1.19% of the tyrosine reached the adjacent arteries directly. From these investigations it is concluded that molecules with a molecular weight of approximately 6000 can be transferred directly from veins to arteries at the ovarian pedicle, and the efficiency of this exchange does not only depend on molecular size.     

N-cadherin在卵巢癌中的表达及其临床病理意义

目的:探讨N-cadherin在人类卵巢癌组织中的表达及其临床-病理意义。方法:采用免疫组织化学染色法检测281例卵巢癌患者肿瘤组织中N-cadherin的表达,并分析其与患者临床病理特征之间的关系。结果:N-cadherin在卵巢癌原发灶中的表达显著低于配对的转移灶(P=0.018);卵巢癌组织中N-cadherin的表达与患者FIGO分期(P=0.034)、组织学类型(P0.001)、肿瘤分级(P=0.004)均显著相关。结论:N-cadherin高表达更多见于进展期(FIGOⅡ-Ⅳ)卵巢癌、高级别浆液性癌及高级别卵巢癌,可能与卵巢癌细胞的侵袭及迁移能力呈正相关,对判断卵巢癌的生物学行为具有重要的参考价值。     

卵巢上皮性癌中干扰素介导的跨膜蛋白1的表达意义

目的:探讨干扰素介导的跨膜蛋白1(Interferon-induced transmembrane protein 1,IFITM1)基因在卵巢上皮性癌中表达的相关性及其意义。方法:应用Western blotting检测正常卵巢、卵巢良性肿瘤、卵巢交界性肿瘤和卵巢上皮性癌组织中IFITM1蛋白表达。免疫组织化学检测12例正常卵巢、21例卵巢良性肿瘤、18例卵巢交界性肿瘤和85例卵巢上皮性癌组织中IFITM1的蛋白表达,同时分析IFITM1表达状况与临床病理因素之间的相关性。结果:Western blotting显示卵巢上皮性癌和卵巢交界性肿瘤中IFITM1表达水平明显高于正常卵巢组织和卵巢良性肿瘤。免疫组化显示在正常卵巢组织中IFITM1阳性表达率为41.7%(5/12),在卵巢良性肿瘤组织中71.4%(15/21),在卵巢交界性肿瘤组织中为72.2%(13/18),在卵巢上皮性癌中为77.6%(66/85),IFITM1蛋白表达强度在正常卵巢、良性卵巢肿瘤、交界性卵巢肿瘤、上皮性卵巢癌间的比较有统计学意义(P0.05)。IFITM1蛋白表达与病理类型、肿瘤分化程度、肿瘤FIGO分期有关(P0.05),与淋巴结转移、腹水无明显相关性。化疗敏感组和耐药组的IFITM1表达强度间差异有统计学意义(P0.05)。结论:IFITM1在正常卵巢、卵巢良性肿瘤、卵巢交界性肿瘤和卵巢上皮性癌组织中的表达依次升高,并与卵巢癌以铂类为基础的化疗耐药性产生有相关性,为进一步研究IFITM1在卵巢癌诊治及化疗中的应用前景提供依据。     

Prostaglandins F in uterine and ovarian venous plasma from nonpregnant and pregnant ewes collected by cannulation

Periodic collections of uterine venous blood were obtained from three nonmated, three pregnant and two mated but nonpregnant ewes in which uterine veins were cannulated with polyvinyl tubing on day 11 postestrus. Frequent sampling was achieved in three of these ewes with additional cannulae in the ovarian veins. Blood samples were collected at 3-hr intervals from 0600 on day 12 to 1800 on day 13 and then at 6-hr intervals through day 15. On day 13, three additional samples at 30-min intervals were collected between 1400 and 1530. Prostaglandins F (PGF) in plasma were quantified by radioimmunoassay.     

山东省网翅蝗属一新种(直翅目,蝗总科,网翅蝗科)

记述了采自中国山东省网翅蝗科的1新种,黄条网翅蝗Arcyptera flavivittata sp.nov..模式标本保存于山东农业大学植物保护学院,泰安.     

Comparative analysis of functions of cow and reindeer female reproductive organs: Progesterone content in vessels of reproductive organs

Progesterone content in blood from paired ovarian and uterine veins as well as from jugular veins of cows and reindeers was studied in the estrous cycle lutein phase and at the earlier stages of pregancy. In the both species, maximal progesterone concentration was detected in blood from vein of the ovary carrying corpus luteum (p < 0.001). In cows, a higher hormone concentration, as compared with jugular vein, has also been determined in vein of the uterus horn closest to ovary with corpus luteum (p < 0.01). In reindeers, blood from all studied vessels of reproductive organs had the progesterone concentration that was statistically significantly higher (p < 0.001) than that from jugular vein. In cows, progesterone concentration in blood from the ovarian vein was found to be higher when corpus luteum was located on the right ovary (p < 0.05) as compared with left-side corpus luteum location. No functional asymmetry of ovaries was revealed in reindeers. A possible role of mechanisms of the hormone local transport between ovary and uterus in adaptation of ruminants to reproduction under Nordic conditions is discussed.     

Local exchange of oxytocin from the ovarian vein to ovarian arteries in sheep

Local transfer of 125I-labeled oxytocin from the ovarian vein to arteries supplying the ovary, the oviduct, and the tip of the uterine born has been investigated. In five sheep, 10 infusions of 125I-oxytocin over a period of 1 h were performed, and the concentration of labeled polypeptide in the peripheral plasma was compared to ovarian arterial plasma. During 2 consecutive infusions into each animal's ovarian vein, blood was collected simultaneously from the following sites: ovarian branch of the ovarian artery (OBOA), tubal branch of the ovarian artery (TBOA), uterine branch of the ovarian artery (UBOA), and from the jugular vein. In all experiments the concentration of 125I-oxytocin in ovarian arterial plasma was higher than in peripheral plasma. The ratio of ovarian artery/jugular vein for 125I-oxytocin was: OBOA 2.8, TBOA 1.8, UBOA 1.6. Based on a 4 ml/min blood flow through ovarian arteries supplying ovary, oviduct, and the tip of the uterine horn, the local transfer of the total amount of oxytocin infused was estimated to be about 1% (range: 0.1-4.4%). Analysis of variance did not reveal significant differences in the exchange ratios between OBOA, TBOA, and OBOA. However, the variances within these groups are significant, presumably because of anatomical variation in the degree of surface contact area between arteries and veins at the ovarian pedicle. It is concluded that polypeptides are locally recirculated to ovaries, oviduct, and the tip of the uterine horn in a higher concentration than is supplied by peripheral blood. This could provide a mechanism for local distribution and concentration of the ovarian peptides that regulate reproductive function.     

Prostaglandins F in uterine and ovarian venous plasma from nonpregnant and pregnant ewes collected by cannulation.

Periodic collections of uterine venous blood were obtained from three nonmated, three pregnant and two mated but nonpregnant ewes in which uterine veins were cannulated with polyvinyl tubing on day 11 postestrus. Frequent sampling was achieved in three of these ewes with additional cannulae in the ovarian veins. Blood samples were collected at 3-hr intervals from 0600 on day 12 to 1800 on day 13 and then 6-hr intervals through day 15. On day 13, three additional samples at 30-min intervals were collected between 1400 and 1530. Prostaglandins F (PGF) in plasma were quantified by radioimmunoassay. On day 12, one ewe in each group had at least one measurement which suggested an increased rate of release of PGF into the uterine vein. Seven of eight ewes on day 13 appeared to have increased rates of release of PGF from the uterus between 0900 and 1500. The highest level measured in each ewe during this period ranged from 2.7 to 11 ng per milliliter. Concentrations of PGF in ovarian venous plasma in two of three ewes were positively correlated (P less than .05) with concentrations of PGF in uterine venous plasma (r equals .64 in each ewe). No evidence was obtained that pregnant and nonpregnant ewes differ in rate or pattern of release of PGF from the uterus into the uterine vein on days 12 and 13. Comparisons could not be made with confidence concerning PGF either in uterine veins on days 14 and 15 or in ovarian veins on all days due to limited number of observations.