Role of Intracellular pH in Proliferation, Transformation, and Apoptosis

Both cellular proliferation and apoptosis (programmed cell death) have been claimed to be modulated, perhaps even triggered by, changes in intracellular pH. In this review, we summarize the evidence that gave rise to these hypotheses. To facilitate a critical appraisal of the existing data, we briefly review the main pathways involved in cytosolic pH homeostasis and their regulation by mitogens and by apoptosis-inducing agents. The information available at present suggests that cytosolic pH plays a permissive role in cellular growth and proliferation, but is neither a trigger nor an essential step in the mitogenic signal transduction cascade. Concerning apoptosis, it is clear that lowering the pH in vitro can activate DNase II. However, the evidence linking cytosolic acidification with DNA degradation in vivois presently not convincing. We conclude that the cytosolic pH, an essential physiological parameter that is tightly controlled by multiple, complementary, or redundant systems, is unlikely to play a role in signalling either cell growth or death.     

Loading pyranine via purinergic receptors or hypotonic stress for measurement of cytosolic pH by imaging

Although used extensively for the measurement of intracellularpH, derivatives of fluorescein such as2',7'-bis(2-carboxyethyl)-5(6)-carboxyfluorescein (BCECF)have suboptimal sensitivity and can generate toxic photoproducts. Theselimitations can be overcome using the pH-sensitive fluorescent dye8-hydroxypyrene-1,3,6-trisulfonic acid (pyranine), which has improvedspectroscopic properties. However, the use of pyranine has been limitedby the difficulties encountered in delivering this highly hydrophilicdye to the cell interior. We describe a strategy for intracellulardelivery of pyranine based on the reversible activation of purinergicP_2x7 receptors, which allow permeation of the dye into otherwise intact cells. When loaded intoJ774 or RAW cells by this method, pyranine is not only more sensitivethan BCECF (the dynamic range is ~7-fold greater), but is retainedbetter and is less toxic. Pyranine was distributed throughout thecytosol but was not detectable in endomembrane compartments. Repeatedillumination resulted in blebbing and loss of functional responsivenessof cells loaded with BCECF, whereas comparably irradiated cells loadedwith pyranine remained healthy and responsive. Pyranine can also beloaded into cells not expressing P_2x7 receptors by brief exposureto a hypotonic solution. The properties of cells labeled by this methodare similar to those loaded via purinergic receptors and comparefavorably with those of BCECF-loaded cells. Pyranine thus provides auseful alternative to fluorescein derivatives for the measurement ofintracellular pH, particularly when using the high excitationintensities required for microscopic digital imaging.

     

vvd is required for light adaptation of conidiation-specific genes of Neurospora crassa, but not circadian conidiation

con-10 and con-6 are two of the conidiation (con) genes of Neurospora crassa that were identified based on their preferential expression during macroconidiophore development. They are also regulated by several other environmental stimuli independent of development, including a transient induction by light. We identified an allele of vivid (vvd) in a mutant screen designed to obtain strains with altered expression of con-10. vvd mutants display enhanced carotenoid pigmentation in response to light. In addition, con-10 and con-6 show a heightened response to photoinduction. We tested the function of the light-responsive circadian clock in the vvd mutant and found no major defect in the circadian rhythm of conidiation or light regulation of a key clock component, frequency (frq). We conclude that vvd is primarily involved in a process of light-dependent gene repression, called light adaptation. Although a number of gene products are known to control light induction in fungi, vvd is the first gene shown to have a role in adaptation to constant light.     

Topological analysis of NHE1, the ubiquitous Na+/H+ exchanger using chymotryptic cleavage

Proteases,glycosidases, and impermeant biotin derivatives were used incombination with antibodies to analyze the subcellular distribution andtransmembrane disposition of theNa⁺/H⁺exchanger NHE1. Both native human NHE1 in platelets and epitope-tagged rat NHE1 transfected into antiport-deficient cells were used for thesestudies. The results indicated that1) the entire population ofexchangers is present on the surface membrane of unstimulated platelets, ruling out regulation by recruitment of internal stores ofNHE1; 2) the putative extracellularloops near the NH₂ terminus areexposed to the medium and contain all the N- andO-linked carbohydrates;3) by contrast, the putativeextracellular loops between transmembrane domains 9-10 and11-12 are not readily accessible from the outside and may befolded within the protein, perhaps contributing to an aqueous iontransport pathway; 4) the extreme COOH terminus of the protein was found to be inaccessible toextracellular proteases, antibodies, and other impermeant reagents,consistent with a cytosolic localization; and5) detachment of ~150 amino acidsfrom the NH₂-terminal end of theprotein had little effect on the transport activity of NHE1.

     

Genetic characterization of the bovine leukaemia inhibitory factor (LIF) gene: isolation and sequencing, chromosome assignment and microsatellite analysis

The bovine leukaemia inhibitory factor was isolated from a phage library and sequences for the gene, in addition to 1213bp of 5' and 432bp of 3' sequences, were obtained and compared with other mammalian leukaemia inhibitory factor genes. Comparisons indicated amino acid homologies ranging from 89·6% to 77·2% with the human and mouse homologues, respectively. Analysis of 500bp of 5' regulatory regions indicated homologies ranging from 83·6% to 74·4% with the corresponding human and sheep sequences, respectively. Additionally, bovine leukaemia inhibitory factor-specific primers were prepared, and a panel of bovine × hamster somatic cell lines were analysed by the polymerase chain reaction (PCR). Data indicated 93% concordance of leukaemia inhibitory factor with aldehyde dehydrogenase 2 located on bovine chromosome 17, and concordance of 81% with myelin basic protein situated on bovine chromosome 24. Southern analysis of selected hybrids confirmed the PCR results, thus conclusively assigning the bovine leukaemia inhibitory factor gene to chromosome 17. Sequence analysis also revealed a microsatellite in intron 2 of the bovine leukaemia inhibitory factor. Analysis of this region by PCR in 22 unrelated Bos taurus and 19 unrelated Bos indicus cattle detected nine different alleles. Polymorphic information content values were 0·53 and 0·80 in B. taurus and B. indicus , respectively. Additionally, the same leukaemia inhibitory factor primers successfully detected allelic variants at this locus in Bos javanicus , Bos guarus and Bison bison but not in Odocoileus virginianus .     

Localization of endogenous and recombinant Na+-driven anion exchanger protein NDAE1 from Drosophila melanogaster

Na⁺-dependent Cl/HCOexchange activity helps maintain intracellular pH (pH_i)homeostasis in many invertebrate and vertebrate cell types. Ourlaboratory cloned and characterized a Na⁺-dependentCl/HCO exchanger (NDAE1) fromDrosophila melanogaster (Romero MF, Henry D, Nelson S, HartePJ, and Sciortino CM. J Biol Chem 275:24552-24559, 2000). In the present study we usedimmunohistochemical and Western blot techniques to characterize thedevelopmental expression, subcellular localization, and tissue distribution of NDAE1 protein in D. melanogaster. We haveshown that a polyclonal antibody raised against the NH₂terminus of NDAE1 (CWR57) recognizes NDAE1 electrophysiologicallycharacterized in Xenopus oocytes. Moreover, our resultsbegin to delineate the NDAE1 topology, i.e., both the NH₂and COOH termini are intracellular. NDAE1 is expressed throughoutDrosophila development in the central and peripheral nervoussystems, sensilla, and the alimentary tract (Malpighian tubules, gut,and salivary glands). Coimmunolabeling of larval tissues with NDAE1antibody and a monoclonal antibody to theNa⁺-K⁺-ATPase -subunit revealed that themajority of NDAE1 is located at the basolateral membranes of Malpighiantubule cells. These results suggest that NDAE1 may be a keypH_i regulatory protein and may contribute to basolateralion transport in epithelia and nervous system of Drosophila.

     

Osmotic Stimulation of the Na+/H+ Exchanger NHE1: Relationship to the Activation of Three MAPK Pathways

The Na⁺/H⁺ exchanger (NHE) becomes activated by hyperosmolar stress, thereby contributing to cell volume regulation. The signaling pathway(s) responsible for the shrinkage-induced activation of NHE, however, remain unknown. A family of mitogen-activated protein kinases (MAPK), encompassing p42/p44 Erk, p38 MAPK and SAPK, has been implicated in a variety of cellular responses to changes in osmolarity. We therefore investigated whether these kinases similarly signal the hyperosmotic activation of NHE. The time course and osmolyte concentration dependence of hypertonic activation of NHE and of the three sub-families of MAPK were compared in U937 cells. The temporal course and dependence on osmolarity of Erk and p38 MAPK activation were found to be similar to that of NHE stimulation. However, while pretreatment of U937 cells with the kinase inhibitors PD98059 and SB203580 abrogated the osmotic activation of Erk and p38 MAPK, respectively, it did not prevent the associated stimulation of NHE. Thus, Erk1/2 and/or p38 MAPK are unlikely to mediate the osmotic regulation of NHE. The kinetics of NHE activation by hyperosmolarity appeared to precede SAPK activation. In addition, hyperosmotic activation of NHE persisted in mouse embryonic fibroblasts lacking SEK1/MKK4, an upstream activator of SAPK. Moreover, shrinkage-induced activation of NHE still occurred in COS-7 cells that were transiently transfected with a dominant-negative form of SEK1/MKK4 (SEK1/MKK4-A/L) that is expected to inhibit other isoforms of SEK as well. Together, these results demonstrate that the stimulation of NHE and the activation of Erk, p38 MAPK and SAPK are parallel but independent events. Received: 27 November 2000/Revised: 20 March 2001