A second-generation linkage map of the sheep genome

A genetic map of Ovis aries (haploid n = 27) was developed with 519 markers (504 microsatellites) spanning ∼3063 cM in 26 autosomal linkage groups and 127 cM (female specific) of the X Chromosome (Chr). Genotypic data were merged from the IMF flock (Crawford et al., Genetics 140, 703, 1995) and the USDA mapping flock. Seventy-three percent (370/504) of the microsatellite markers on the map are common to the USDA-ARS MARC cattle linkage map, with 27 of the common markers derived from sheep. The number of common markers per homologous linkage group ranges from 5 to 22 and spans a total of 2866 cM (sex average) in sheep and 2817 cM in cattle. Marker order within a linkage group was consistent between the two species with limited exceptions. The reported translocation between the telomeric end of bovine Chr 9 (BTA 9) and BTA 14 to form ovine Chr 9 is represented by a 15-cM region containing 5 common markers. The significant genomic conservation of marker order will allow use of linkage maps in both species to facilitate the search for quantitative trait loci (QTLs) in cattle and sheep. Received: 20 September 1992 / Accepted: 18 November 1997     

Nitric oxide control of lower vertebrate blood vessels by vasomotor nerves

In mammals, much is understood about the endothelial and neural NO control mechanisms in the vasculature. In contrast, NO control of blood vessels in lower vertebrates is poorly understood, with the majority of research focusing on the presence of an endothelial NO system; however, its presence remains controversial. This study examined the mechanisms by which NO regulates the large blood vessels of non-mammalian vertebrates. In all species examined, the arteries and veins contained a plexus of NOS-positive perivascular nerves that included nerve bundles and fine, varicose nerve terminals. However, in the large arteries and veins of various species of fishes and amphibians, no anatomical evidence was found for endothelial NOS using both NADPH-diaphorase and eNOS immunohistochemistry. In contrast, perinuclear NOS staining was readily apparent in blue-tongue lizard, pigeon and rat, which suggested that eNOS first appeared in reptiles. Physiological analysis of NO signalling in the vascular smooth muscle of short-finned eel and cane toad could not find any evidence for endothelial NO signalling. In contrast, it appears that activation of the nitrergic vasomotor nerves is responsible for NO control of the blood vessels.     

Conserved regulation of MAP kinase expression by PUF RNA-binding proteins

Mitogen-activated protein kinase (MAPK) and PUF (for Pumilio and FBF [fem-3 binding factor]) RNA-binding proteins control many cellular processes critical for animal development and tissue homeostasis. In the present work, we report that PUF proteins act directly on MAPK/ERK-encoding mRNAs to downregulate their expression in both the Caenorhabditis elegans germline and human embryonic stem cells. In C. elegans, FBF/PUF binds regulatory elements in the mpk-1 3′ untranslated region (3′ UTR) and coprecipitates with mpk-1 mRNA; moreover, mpk-1 expression increases dramatically in FBF mutants. In human embryonic stem cells, PUM2/PUF binds 3′UTR elements in both Erk2 and p38α mRNAs, and PUM2 represses reporter constructs carrying either Erk2 or p38α 3′ UTRs. Therefore, the PUF control of MAPK expression is conserved. Its biological function was explored in nematodes, where FBF promotes the self-renewal of germline stem cells, and MPK-1 promotes oocyte maturation and germ cell apoptosis. We found that FBF acts redundantly with LIP-1, the C. elegans homolog of MAPK phosphatase (MKP), to restrict MAPK activity and prevent apoptosis. In mammals, activated MAPK can promote apoptosis of cancer cells and restrict stem cell self-renewal, and MKP is upregulated in cancer cells. We propose that the dual negative regulation of MAPK by both PUF repression and MKP inhibition may be a conserved mechanism that influences both stem cell maintenance and tumor progression.     

Ethylene-Stimulated Nutations Do Not Require ETR1 Receptor Histidine Kinase Activity

Ethylene influences the growth and development of plants through the action of receptors that have homology to bacterial two-component receptors. In bacteria these receptors function via autophosphorylation of a His residue in the kinase domain followed by phosphotransfer to a conserved Asp residue in a response regulator protein. In Arabidopsis, two of the five receptor isoforms are capable of His kinase activity. However, the role of His kinase activity and phosphotransfer is unclear in ethylene signaling. A previous study showed that ethylene stimulates nutations of the hypocotyl in etiolated Arabidopsis seedlings that are dependent on the ETR1 receptor isoform. The ETR1 receptor is the only isoform in Arabidopsis that contains both a functional His kinase domain and a receiver domain for phosphotransfer. Therefore, we examined the role that ETR1 His kinase activity and phosphotransfer plays in ethylene-stimulated nutations.Key Words: ethylene, nutations, signal transduction, receptors, histidine kinase, phosphotransfer, two component signallingThe gaseous plant hormone ethylene has a role in a variety of physiological events in higher plants such as seed germination, abscission, senescence, fruit ripening, and growth regulation.¹ In etiolated Arabidopsis seedlings, ethylene causes reduced growth of the hypocotyl and root, increased radial expansion of the hypocotyl, and increased tightening of the apical hook.^2,3Previous studies have identified components in the ethylene signaling pathway and led to an inverse-agonist model for signal transduction.^4,5 According to this model, responses to ethylene are mediated by a family of five receptors (ETR1, ERS1, ETR2, EIN4, ERS2) in Arabidopsis that have homology to bacterial two-component receptors.^6–9 In bacterial systems, two-component receptors transduce signal via the autophosphorylation of a His residue in the kinase domain, followed by the transfer of phosphate to a conserved Asp residue in the receiver domain of a response regulator protein.¹⁰ The ethylene receptors of plants can be divided into two subfamilies based on sequence homology in the ethylene-binding domains.¹¹ ETR1 and ERS1 belong to subfamily I, contain all amino acid residues needed for His kinase activity,^6,12 and show His kinase activity in vitro.^13,14 ETR2, EIN4, and ERS2 belong to subfamily II, contain degenerate His kinase domains^7,9 and have Ser/Thr kinase activity in vitro.¹⁴ ERS1 shows both His and Ser/Thr kinase activities in vitro depending on the assay conditions used.¹⁴ While the kinase domain of ETR1 appears to be required for signaling,¹⁵ kinase activity is not.^15–17 It is unclear whether or not histidine kinase activity is involved in ethylene signaling, although, this activity might be involved in growth recovery after ethylene removal.¹⁷Recently, high-resolution, time-lapse imaging revealed that prolonged treatment with ethylene stimulates nutational bending of etiolated Arabidopsis hypocotyls.¹⁸ Nutations are oscillatory bending movements caused by localized differential growth¹⁹ that were originally termed “circumnutations”.²⁰ Nutations have been posited to be important for seedlings to penetrate through the soil²⁰ and thus could be critical for seedling survival. In support of this hypothesis, nutations of rice roots have been reported to increase soil penetration.²¹Mutational analysis revealed that many of the known ethylene signaling components including CTR1, EIN2, EIN3 and EIL1 are involved in signaling leading to ethylene-stimulated nutations.¹⁸ Surprisingly, loss-of-function mutations in ETR1 eliminated ethylene-stimulated nutations while combinatorial loss-of-function mutations in the other four receptor isoforms led to constitutive nutations in air.¹⁸ These results support a model where all the receptors are involved in ethylene-stimulated nutations but the ETR1 receptor is required for and has a contrasting role from the other receptor isoforms in this nutation phenotype. Since the ETR1 receptor is the only receptor isoform that contains both a functional His-kinase domain and a receiver domain,^6,13,14 the roles of His kinase activity and phosphorelay in the nutation phenotype were examined in the current study.Previous work showed that the nutation phenotype in etr1-7 loss-of-function mutants could be rescued with a wild-type, genomic ETR1 transgene.¹⁸ Etr1-7 mutants transformed with a kinase-inactivated genomic ETR1 transgene (gETR1 (G₂)) where the two conserved glycines in the G₂ box of the histidine kinase domain (G545, G547) were changed to alanines were examined to determine if ETR1 His kinase activity is required for ethylene-stimulated nutations. This construct lacks histidine autophosphorylation in vitro.²² Figure 1 shows that ethylene stimulates nutations in etr1-7 gETR1(G₂) seedlings. The period of these nutations was 4.7 ± 1.5 h which is similar to values obtained previously for wild-type seedlings (4.7 ± 1h) and somewhat longer than etr1-7 seedlings transformed with wild-type, genomic ETR1 (3.2 ± 0.6 h). However, the amplitude of these nutations (3.7 ± 1.0°) was approximately half that of nutations previously observed in wild-type seedlings (9.1 ± 6.0°) as well as etr1-7 seedlings transformed with wild-type, genomic ETR1 (8.2 ± 3.6°). This suggests that ETR1 histidine kinase activity is not required for ethylene-stimulated nutations but might have a role in modulating nutation amplitudes.Open in a separate windowFigure 1Ethylene stimulates nutations of etr1-7 seedlings transformed with a kinase-inactivated ETR1 transgene. The hypocotyl angles for four etr1-7 mutants transformed with a kinase-inactivated genomic ETR1 transgene (gETR1(G₂)) are shown. Transformants were obtained from Eric Schaller and have been described previously.²² In this and the following figure, etiolated Arabidopsis seedlings were imaged from the side at 15 min intervals while growing along a vertically orientated agar plate and the hypocotyl angle measured as described previously.¹⁸ Black and gray lines are used to help distinguish the movements of individual seedlings. All seedlings were grown in the presence of 5 µM AVG to block biosynthesis of ethylene by the seedlings. Seedlings were grown in air for 2 h prior to treatment with 10 µL L⁻¹ ethylene (Open in a separate window).To determine whether phosphotransfer through the receiver domain of ETR1 is required for the nutation phenotype, seedlings deficient in ethylene receptor isoforms containing a receiver domain (ETR1, ETR2, EIN4) were transformed with a mutant ETR1 transgene lacking the conserved Asp₆₅₉ required for phosphotransfer (getr1-[D]). Previous work showed that etr1-6 etr2-3 ein4-4 triple loss-of-function mutant seedlings failed to nutate and this nutation phenotype could be rescued when these mutants were transformed with wild-type, genomic ETR1 transgene.¹⁸ Similarly, transformation of the etr1-6 etr2-3 ein4-4 triple mutants with getr1-[D] rescued the nutation phenotype in most seedlings observed (Fig. 2). However, some seedlings (four of the eleven observed) failed to nutate. The reason for this variable rescue is unclear but could reflect differences in expression levels of the mutant transgene in individual plants. Alternatively, this variable rescue could reflect functional differences between the mutant and wild-type transgene suggesting a modulating role for phosphotransfer through the receiver domain of ETR1. Two independent lines were observed with similar results. Of those that did nutate, the period of nutations was 5.0 ± 1.2 h and the amplitude 7.6 ± 3.8° which is similar to values obtained previously for wild-type plants as well as plants transformed with a wild-type, genomic ETR1 transgene.¹⁸Open in a separate windowFigure 2Ethylene stimulates nutations of etr1-6 etr2-3 ein4-4 seedlings transformed with an ETR1 transgene mutated at Asp₆₅₉. The hypocotyl angles from seven etr1-6 etr2-3 ein4-4 triple mutants transformed with an ETR1 transgene mutated at Asp₆₅₉ (getr1[D]) are shown in two panels. One seedling in (A) (black) had no measurable nutations while one in (B) (black) had very small nutations.Conclusions from this and the previous study are that the ETR1 receptor has a unique role in ethylene-stimulated nutations. However, this role does not require either histidine kinase activity or phosphotransfer through the receiver domain of ETR1.     

Effect of repeated apoA-IMilano/POPC infusion on lipids, (apo)lipoproteins,and serum cholesterol efflux capacity in cynomolgus monkeys

MDCO-216, a complex of dimeric recombinant apoA-IMilano (apoA-IM) and palmitoyl-oleoyl-phosphatidylcholine (POPC), was administered to cynomolgus monkeys at 30, 100, and 300 mg/kg every other day for a total of 21 infusions, and effects on lipids, (apo)lipoproteins, and ex-vivo cholesterol efflux capacity were monitored. After 7 or 20 infusions, free cholesterol (FC) and phospholipids (PL) were strongly increased, and HDL-cholesterol (HDL-C), apoA-I, and apoA-II were strongly decreased. We then measured short-term effects on apoA-IM, lipids, and (apo)lipoproteins after the first or the last infusion. After the first infusion, PL and FC went up in the HDL region and also in the LDL and VLDL regions. ApoE shifted from HDL to LDL and VLDL regions, while ApoA-IM remained located in the HDL region. On day 41, ApoE levels were 8-fold higher than on day 1, and FC, PL, and apoE resided mostly in LDL and VLDL regions. Drug infusion quickly decreased the endogenous cholesterol esterification rate. ABCA1-mediated cholesterol efflux on day 41 was markedly increased, whereas scavenger receptor type B1 (SRB1) and ABCG1-mediated effluxes were only weakly increased. Strong increase of FC is due to sustained stimulation of ABCA1-mediated efflux, and drop in HDL and formation of large apoE-rich particles are due to lack of LCAT activation.     

Nitric oxide and attenuated reflex cutaneous vasodilation in aged skin

Thermoregulatory cutaneous vasodilation is diminished in the elderly. The goal of this study was to test the hypothesis that a reduction in nitric oxide (NO)-dependent mechanisms contributes to the attenuated reflex cutaneous vasodilation in older subjects. Seven young (23 +/- 2 yr) and seven older (71 +/- 6 yr) men were instrumented with two microdialysis fibers in the forearm skin. One site served as control (Ringer infusion), and the second site was perfused with 10 mM N(G)-nitro-l-arginine methyl ester to inhibit NO synthase (NOS) throughout the protocol. Water-perfused suits were used to raise core temperature 1.0 degrees C. Red blood cell (RBC) flux was measured with laser-Doppler flowmetry over each microdialysis fiber. Cutaneous vascular conductance (CVC) was calculated as RBC flux per mean arterial pressure, with values expressed as a percentage of maximal vasodilation (infusion of 28 mM sodium nitroprusside). NOS inhibition reduced CVC from 75 +/- 6% maximal CVC (CVC(max)) to 53 +/- 3% CVC(max) in the young subjects and from 64 +/- 5% CVC(max) to 29 +/- 2% CVC(max) in the older subjects with a 1.0 degrees C rise in core temperature. Thus the relative NO-dependent portion of cutaneous active vasodilation (AVD) accounted for approximately 23% of vasodilation in the young subjects and 60% of the vasodilation in the older subjects at this level of hyperthermia (P < 0.001). In summary, NO-mediated pathways contributed more to the total vasodilatory response of the older subjects at high core temperatures. This suggests that attenuated cutaneous vasodilation with age may be due to a reduction in, or decreased vascular responsiveness to, the unknown neurotransmitter(s) mediating AVD.     

Utilizing a regulated targeted integration cell line development approach to systematically investigate what makes an antibody difficult to express

Chinese hamster ovary (CHO) cells are conventionally used to generate therapeutic cell lines via random integration (RI), where desired transgenes are stably integrated into the genome. Targeted integration (TI) approaches, which involve integration of a transgene into a specific locus in the genome, are increasingly utilized for CHO cell line development (CLD) in recent years. None of these CLD approaches, however, are suitable for expression of toxic or difficult-to-express molecules, or for determining the underlying causes for poor expression of some molecules. Here we introduce a regulated target integration (RTI) system, where the desired transgene is integrated into a specific locus and transcribed under a regulated promoter. This system was used to determine the underlying causes of low protein expression for a difficult-to-express antibody (mAb-A). Interestingly, we observed that both antibody heavy chain (HC) and light chain (LC) subunits of mAb-A independently contributed to its low expression. Analysis of RTI cell lines also revealed that while mAb-A LC triggered accumulation of intracellular BiP, its HC displayed impaired degradation and clearance. RTI pools, generated by swapping the WT or point-mutant versions of difficult-to-express antibody HC and LC with that of an average antibody, were instrumental in understanding the contribution of HC and LC subunits to the overall antibody expression. The ability to selectively turn off the expression of a target transgene in an RTI system could help to directly link expression of a transgene to an observed adverse effect. © 2018 American Institute of Chemical Engineers Biotechnol. Prog., 35: e2772, 2019.     

Overcoming urban stream syndrome: Trophic flexibility confers resilience in a Hawaiian stream fish

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