New developments in calcium ion channel antagonists - Journal of

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Journal of Medicinal Chemistry J

J

0 Copyright 1983 by the American Chemical Society

June 1983

Volume 26, Number 6

Perspective New Developments in Ca2+Channel Antagonists R. A. Janis*vt and D. J. Trigglet Miles Institute for Preclinical Pharmacology, P.O. Box 1956, New Haven, Connecticut 06509, and Department of Biochemical Pharmacology, School of Pharmacy, State University of New York, Buffalo, New York 14260. Received January 21, 1983

Introduction Despite the 100 years that have elapsed since the discovery by Sidney Ringer of the vital role for Ca2+in the maintenance of cardiac contractility, the messenger function of Ca2+has been appreciated only comparatively recently (reviewed in ref 1-3). This messenger function for Ca2+ (Figure l),a consequence of a critical cellular decision probably made early in the course of evolution,4 is made possible by three key features of cellular Ca2+ regulation: (1) In the resting state the intracellular conM), but it centration of ionized (free) Ca2+is low increases during excitation to between and lob M. (2) There exist within the cell specific Ca2+-bindingproteins with dissociation constants for Ca2+of between and M and which serve as intracellular Ca2+receptors. (3) Within the plasma membrane and intracellular organelles, Ca2+-specificentry, exit, and sequestration processes exist. These processes function both to generate the elevated levels of Ca2+during excitation and to restore and maintain the low intracellular Ca2+levels of the resting state. A schematic representation of cellular Ca2+regulation is shown in Figure 2. Cellular Ca2+is stored in intracellular organelles, including mitochondria (MI) and sarcoplasmic reticulum (SR), by energy-dependent transport proce~ses."~ Ca2+ release, notably from sarcoplasmic reticulum and functionally related structures, plays an important role in stimuli that directly or indirectly mobilize intracellular Ca2+. It is probable that the plasma membrane, at its cytosolic interface, also plays an important role in Ca2+storage and release processes. Although both mitochondria and sarcoplasmicreticulum have significant storage capacities for Ca2+,the cell must, in order to avoid the deleterious consequences of Ca2+overload: ultimately remove Ca2+tc, the extracellular environment. At least two Ca2+ mechanisms are involved, a plasmalemma1 Ca2+ATPase and a Na+-Ca2+exchange process."" The latter derives its cation countertransporting ability from Na+,K+-ATPase and may, according to the ratios of intracellular and extracellular Na+, serve to remove Ca2+ from or introduce Ca2+to the cell. Within the cell, the targets for Ca2+are an homologous group of Ca2+-binding proteins, including parvalbumins, troponin C, and calmodulin, that serve to confer Ca2+sensitivity to mechanMiles Institute for Preclinical Pharmacology. University of New York a t Buffalo.

t State

Table I. Calmodulin-Dependent Events Cellular Events contraction of smooth muscle hormone and neurotransmitter release phospholipid breakdown prostaglandin synthesis cell proliferation cell architecture Ca2+transport

motility axonal transport

Enzyme cyclic nucleotide phosphodiesterase adenylate cyclase phosphorylase b kinase NAD+-kinase

Activation myosin light chain kinase phospholipase A, glycogen synthase kinase

ical, secretory, and metabolic e ~ e n t s . ~ bOf J ~particular importance is calmodulin, since it is highly conserved in structure, has a wide-spread phylogenetic distribution, and has multiple roles in Ca2+-dependentcellular regulation (Table W. Y. Cheung, Ed. Calcium Cell Funct., 1 (1980); 2 (1982); 3 (1983). R. H. Kretsinger, Coord. Chem. Rev., 18, 29 (1976). R. H. Kretsinger, Int. Rev. Cytol., 46, 323 (1971). R. H. Kretsinger, in "Calcium Binding Proteins and Calcium Function", R. H. Wasserman, R. A. Corradino,E. Carafoli,R. H. Kretsinger, D. H. MacLennan, and F. L. Siegel, Eds., North-Holland, Amsterdam, 1977, p 63. G. Fiskum and A. L. Lehninger, Calcium Cell Funct., 2, 39 (1982). E. Carafoli and M. Crompton, Curr. Top. Membr. Transp., 10, 151 (1978). A. M. Katz, "Physiology of the Heart", Raven Press, New York, 1977. A. N. E. Zimmerman and W. C. Hulsmann, Nature (London), 211, 646 (1966). H. J. Schatzmann, Curr. Top. Membr. Tramp., 6, 126 (1975). J. P. Bennett, K. A. McGill, and G. B. Warren, Curr. Top. Membr. Tramp., 14, 127 (1980). R. A. Janis and E. E. Daniel, in "Biochemistry of Smooth Muscle", N. E. Stephens, Ed., University Park Press, Baltimore, 1977, p 653. C. van Breemen, P. Aaronson, and R. Loutzenhiser, Pharrnacol. Reu., 30, 167 (1979). M. P. Blaustein, Rev. Physiol. Pharmacol., 70, 33 (1974). A. K. Grover, C. Y. Kwan, and E. E. Daniel, Am. J.Physiol., 240, C175 (1981). G. DeMaille, Calcium Cell Funct., 2, 111 (1982).

0022-2623183 /1826-0775%01.5O/O ._ . , . 0 1983 American Chemical Society I

- I

~

776 Journal of Medicinal Chemistry, 1983, Vol. 26, No. 6

Perspective

VP K+ Depol

Specific Agonists

Nif . ...

J \

DZ

Ca'+ King of the

ca

FYT

'+

Ca2+/Na+

Messengers

Ca2+t

-Bound

Ca"

Figure 1. Ca2+-king of the messengers (with apologies to cyclic

AMP and cyclic GMP). Resp'anse

Figure 3. Ca2+mobilization in response t o plasma membrane signals. Two types of Ca2+channels are shown, receptor-operated

(ROC) and potential-dependent channels (PDC). Specific agonist-receptor interactions (REC-1,REC-2) can mobilize Ca2+ through ROC or from intracellular sources or may depolarize the membrane and activate the PDC. K+-depolarizingstimuli activate PDC only. Ca2+mobilization may also include regenerative (Ca2+ induced) Ca2+release to amplify the signal for producing the response. VP, Nif, and DZ are verapamil, nifedipine, and diltiazem, respectively. Their site of action, which is probably in the Ca2+channel, is not represented in the figure.

a;n I c(HN ,)N : M~

Figure 2. Schematic representation of cellular Ca2+regulation.

Ca2+storage within the cell is shown in mitochondria (MI) and other intracellular loci (Ca2+hJ,including sarcoplasmicreticulum and the internal plasma membrane surface. Ca2+entry, as discussed in the text, can occur through receptor-operated and potential-dependentchannels, as well as through the Na+channel. Intracellular Ca2+levels are regulated through the operation of membrane pumps, including Ca2+-ATPaseand a Na+/Ca2+ countertransport. The functions of intracellular Ca2+are mediated through Ca2+binding proteins, notably calmodulin (CM),shown in cytosolic and membrane-associatedstates. Reproduced from ref 56.

To complement the several storage and efflux processes for Ca2+there exist several influx pathways. Although Ca2+ can enter the cell through a "leak" pathway (unstimulated) and as a minor contributor to the fast inward Na+ current,21it has been proposed that the two major types of Ca2+entry pathways are those that have been designated potential-dependent (PDC) and receptor-operated (ROC) channel^.^^^^^ Potential-dependent channels have been defined as those activated by membrane depolarization (electrical or elevated K+), while receptor-operated channels are those associated with membrane receptors and are activated by specific agonist-receptor interaction. It is not known if the channels themselves are different structures or if the association of ligand receptors with PDC changes their voltage dependence and sensitivity to channel an(16) W.-Y. Cheung, Science, 207, 19 (1980). (17) A. R. Means and J. R. Dedman, Nature (London),285, 73 (1980). (18) W. Y. Cheung, Ed. Calcium Cell Fuunct., 1 (1980). (19) Reu.. . , A. R. Means. J. S. Tash. and T. G. Chafouleas., Phvsiol. 62, 1 (1982). (20) C. B. Klee, T. H. Crouch, and P. G. Richman, Annu. Rev. Biochem., 49, 489 (1980). (21) P. F. Baker and H. G. Glitach, Philos. Trans. R. SOC. London, Ser. B , 270, 389 (1975). (22) T. B. Bolton, Physiol. Revs., 59, 607 (1979). (23) K. D. Meisheri, 0. Hwang, and C. van Breemen,J. Membr. Biol., 59, 19 (1981).

ff3

a;ncl I

(CHZhNMe2

Trifluoperazine

Chlorpromazine

w7

Dibucaine

tl R 24574

Figure 4. Structure of calmodulin antagonists, including a

generalized structure. tagonists and makes them ROC. In principle, Ca2+mobilization during cellular excitation may be initiated from both extracellular and intracellular sources (Figure 3), the relative extent of which will depend on several factors, including the tissue, stimulant, species, the environment of the Ca2+channels, and the effect of other Ca2+regulating mechanisms. These processes of Ca2+regulation at the cellular level are paralleled by Ca2+regulation at the organismic level, where body Ca2+,total and plasma, is regulated by a triumvirate of agents, vitamin D, calcitonin, and parathyroid hormone, serving to regulate Ca2+entry, Ca2+storage, and Ca2+excretion.24 Ca2+Antagonists The ubiquitous role of Ca2+in cell regulation and the diversity of processes controlling cellular Ca2+concentration indicate the importance of identification of the sources and routes of Ca2+mobilization. One approach is through the use of agents that may selectively antagonize the pathways of Ca2+utilization. (24) H. De Luca, Biochem. SOC.Trans., 10, 147 (1982).

Journal of Medicinal Chemistry, 1983, Vol. 26, No. 6 777

Perspective

Table 11. Therapeutic Indications for Caz+ Channel Antagonists Verapamil (R=H) D600 (R=MeO)

Prenylamine

Fendiline Nifedipine

CH,CH,NMe,

Terodiline

Diltiazem

Current Uses angina: vasospastic, unstable a t rest, and chronic stable supraventricular tachycardia ventricular tachyarrhythmia atrial flutter and fibrillation hypertension Possible Future Uses cerebral insufficiency and vasospasm pulmonary hypertension asthma premature labor primary dysmenorrhea, myometrial hyperactivity myocardial ischemia and failure cardiac preservation intestinal spasm peripheral vascular disease esophageal motor disorders, achlasia

structure for calmodulin antagonists as shown in Figure 4. The Ca2+channel antagonists (Figure 5) resemble the Figure 5. Structure of Ca2+channel antagonists. calmodulin antagonists in that they are also a diverse group of molecular structures. Unlike the calmodulin antagoThere is an abundance of structures possessing to some nists, however, the Ca2+channel antagonists are highly degree the ability to inhibit Ca2+-dependent potent, exhibit Ca2+channel antagonism as their principal For most of these structures, however, their ability to pharmacologicalproperty, and possess defined structureantagonize Ca2+-mediatedprocesses is probably indirect activity relationships, including stereoselectivity. The and, in any event, is clearly secondary to other and better remainder of this review will focus on this group of Ca2+ defined pharmacological activities. However, considerable antagonists. attention has been paid in recent years to two major groups Ca2+ Channel Antagonists. The drugs currently of compounds-the calmodulin antagonists (Figure 4) and available in North America, verapamil, nifedipine, dilthe Ca2+channel antagonists (Figure 5). tiazem, and lidoflazine, have a number of therapeutic inCalmodulin Antagonists. Both groups of compounds dications (Table II).34-36These drugs are the first anare characterized by significant heterogeneity of chemical tianginal agents introduced to the United States within structure, which may suggest multiple sites and mechathe last decade that have the potential of becoming drugs nisms of action. However, for the compounds depicted in of choice for most patients with angina. The description Figure 4, it is apparent that their ability to interact with of these agents, variously referred to as Ca2+antagonists, calmodulin is dominated largely by hydrophobic interacCaZf channel antagonists, slow channel blockers, or Ca2+ t i o n ~ , ~ consistent ’-~~ with their interaction a t a nonpolar entry blockers, owes much to the original investigations site on calmodulin exposed during the prerequisite step of Fleckenstein who first observed that verapamil and of Ca2+binding.31 Neither binding to calmodulin nor prenylamine mimic the cardiac effects of Ca2+withdrawinhibition of calmodulin-dependent phosphodiesterase by al.37 Subsequent studies showed that these and a number the isomers of butaclamol, thiothixene, or flupenthixol of other agents, including nifedipine, fendiline, and per~ ~ ~ ~ ~ ~ consistent with exhibits ~ t e r e o s e l e c t i v i t y , 2observations hexiline, were cardiodepressant and coronary vasodilator a relatively nonspecific mode of interaction with calmodrugs acting in an apparently competitive fashion against dulin and in marked contrast to the stereoselectivity of Ca2+ and served to introduce the principle of specific Ca2+ these same compounds, exhibited at much lower concenSince the original studies antagonism to therapeutics.trations, in inhibiting dopamine receptor binding and with verapamil and prenylamine, a large number of adadenylate cyclase a c t i v a t i ~ n Nonetheless, . ~ ~ ~ ~ ~ hydro~~~~~~ ditional structures have joined this class of Ca2+antagophobicity is not the sole determinant of calmodulin annists (Figure 5 ) , and it is clear that this group of comtagonism, and Weiss and his colleaguesB suggest a general pounds is neither structurally nor pharmacologically homogeneous.”,Thus, Fleckensteina (see also ref 41 and 43) has divided compounds into group A (verapamil, D600, L. B. Rosenberger and D. J. Triggle, in “Calcium and Drug BeDridil

Flunorizine ( R = F)

Action”, G. B. Weiss, Ed., Plenum Press, New York, 1978, p 3. D. J. Triggle and V. C. Swamy, Chest (Suppl.), 78, 174 (1980). R. M. Levin and B. Weiss, J.Pharmacol. Exp. Ther., 208,454 (1979). J. A. Norman, A. H. Drummond, and P. Moser, Mol. Pharmacol., 16, 1084 (1979). B. Weiss, W. C. Prozialeck, and T. L. Wallace, Biochem. Pharmacol., 31, 2217 (1982). B. Roufogalis, Calcium Cell Funct., 3, 129 (1983). D. W. La Porte, B. M. Wierman, and D. R. Storm, Biochemistry, 19, 5814 (1980). B. Weiss and T. L. Wallace, Calcium Cell Funct., 1, 330 (1980). B. Weiss, W. Prozialeck, M. Cimino, M. S. Barnette, and T. L. Wallace, Ann. N.Y. Acad. Sci., 356, 319 (1980).

(34) P. D. Henry. in ref 36. D 135. P. H. Stone;E. M. Antman, J. E. Muller, and E. Braunwald, Ann. Int. Med., 93, 886 (1980). S. F. Flaim and R. Zelis, Eds., “Calcium BlockersMechanisms of Action and Clinical Implications”, Urban & Schwarzenberg, Baltimore and Munich, 1982. A. Fleckenstein, Verh. Deutsch. Ges.-Znn. Med., 70,81(1964). A. Fleckenstein, in “Calcium and the Heart”, P. Harris and L. Opie, Eds., Academic Press, London and New York, 1971, p 135. A. Fleckenstein, Annu. Reu. Pharmacol. Toxicol., 17, 149 (1977). A. Fleckenstein, in ref 46, p 59. W. G. Nayler, in ref 49, p 1. R. Rodenkirchen, R. Bayer, and R. Mannhold, Prog. Pharmacol., 5, 9 (1982).

778 Journal of Medicinal Chemistry, 1983, Vol. 26, No. 6 Table 111. Antagonist Activities in Smooth Musclesa system guinea pig ileum

ACh

antagonist

ID,,,M

nifedipine

5x 3 x 10-9 5 x 10-7 2 x 10-7 >10-4